Modifications of Porphyrins and Hydroporphyrins for Their Solubilization in Aqueous Media

The increasing popularity of porphyrins and hydroporphyrins for use in a variety of biomedical (photodynamic therapy, fluorescence tagging and imaging, photoacoustic imaging) and technical (chemosensing, catalysis, light harvesting) applications is also associated with the growing number of methodologies that enable their solubilization in aqueous media. Natively, the vast majority of synthetic porphyrinic compounds are not water-soluble. Moreover, any water-solubility imposes several restrictions on the synthetic chemist on when to install solubilizing groups in the synthetic sequence, and how to isolate and purify these compounds. This review summarizes the chemical modifications to render synthetic porphyrins water-soluble, with a focus on the work disclosed since 2000. Where available, practical data such as solubility, indicators for the degree of aggregation, and special notes for the practitioner are listed. We hope that this review will guide synthetic chemists through the many strategies known to make porphyrins and hydroporphyrins water soluble.

Initial efforts to impart water-solubility relied on the utilization of meso-pyridyl and meso-p-sulfonatophenyl-substituents in (mostly) symmetric porphyrins. These porphyrins were based on Adler syntheses of tetrapyridyl-and tetraphenylporphyrin, followed by quarternization with a suitable alkyl halide or direct sulfonation, respectively. Albeit simple, both methods have drawbacks.
are difficult to translate to β-alkyl-substituted porphyrins, the sulfonation reaction conditions are harsh and therefore incompatible with many hydroporphyrin chromophores or substituents that convey desirable properties onto the porphyrin. This led to the development of a range of alternative methods to impart water-solubility that are mild, selective, and that generate the water-soluble porphyrin derivative late in the synthetic sequence, thus facilitating its isolation and purification.
Rather than attempting to be comprehensive, we aim to present here a tutorial-style review that highlights recent (since ~2000) synthetic strategies. Where data are available, we compare the resulting solubilities, and report on other notable practical considerations. This summary extends a review on water-soluble porphyrins published in the year 2000 [40] that provides a detailed account of the acidbase properties and aggregation behavior of conventional water-soluble porphyrins. A 2014 review on amphiphilic porphyrins by Gryko and co-workers [41] is also available; overlap with this review is minimized and these reviews are thus complementary. Porphyrins linked to sugars, many of which are also water-soluble, have been reported [41][42][43]. We chose not to include them here because glycosylation strategies are frequently not driven by achieving water-solubility but to increase tumor targeting; they were also reviewed in the context of amphiphilic porphyrins [41]. Water-soluble porphyrins conjugated to biomolecules (e.g., oligonucleotides and peptides), appended to functionalities such as cyclodextrans [44], crown ethers [45,46], porphyrin nanoparticles [47][48][49][50], or porphyrins that were solubilized with the help of surfactants or vesicles [51][52][53] are also beyond the scope of this discussion. Likewise, we do not cover the solubilization of expanded porphyrins or most other porphyrinoids.
The review is organized along the charge the solubilization groups introduce: Cationic (amine/ammonium, pyridyl/pyridinium), anionic (sulfonate, phosphonate, carboxylic acid/carboxylate) and neutral (polyethylene glycol (PEG) chains). Each section discusses the examples loosely in increasing order of complexity and the position of the solubilizing group. Three principle strategies for the introduction of solubilizing groups can be distinguished (Scheme 1). Strategy A encompasses the synthesis of a porphyrin macrocycle using building blocks bearing solubilizing groups (protected or not). Strategy B involves the synthesis of a porphyrin macrocycle with precursor functionalities, that can later be manipulated to hydrophilic groups. Strategy C employs synthetic modifications of an already-formed porphyrin to impart water solubility. Scheme 1. Principle strategies toward hydrophilic porphyrin derivatives. prepared a range of water-soluble cationic bacteriochlorin derivatives utilizing the versatile 3,13-dibromo-bacteriochlorin building block 14. The bromo groups are susceptible to a variety of transition metal-mediated C-C bond forming coupling reactions (Scheme 5) [63]. For example, bacteriochlorins 15a-15c were prepared from 14 through a carbonylation → acid chloride reaction with secondary amines. Additionally, reaction of amide salts with 14 in a carbonylation → amidation sequence gave the aminobacteriochlorins 16a and 16b. Sonogashira coupling of 14 with an ethynyl-amine, followed by reduction gave the bacteriochlorin 17 with amine-terminated alkyl chains. Lastly, a variety of secondary amines were employed in a β-formylation → reductive-amination strategy to produce amine-functionalized bacteriochlorins 18a-18e. The resulting amines were amenable to purification by silica gel column chromatography (EtOAc or CH 2 Cl 2 /MeOH/NH 4 OH as eluents). Subsequent N-alkylation of the amines was achieved using standard conditions, and the water-soluble cationic products that precipitated from the CHCl 3 reaction mixtures were isolated by precipitation and centrifugation. Some of these compounds were investigated for their efficacy as antimicrobial photosensitizers [64]. range of water-soluble cationic bacteriochlorin derivatives utilizing the versatile 3,13-dibromobacteriochlorin building block 14. The bromo groups are susceptible to a variety of transition metalmediated C-C bond forming coupling reactions (Scheme 5) [63]. For example, bacteriochlorins 15a-15c were prepared from 14 through a carbonylation → acid chloride reaction with secondary amines. Additionally, reaction of amide salts with 14 in a carbonylation → amidation sequence gave the aminobacteriochlorins 16a and 16b. Sonogashira coupling of 14 with an ethynyl-amine, followed by reduction gave the bacteriochlorin 17 with amine-terminated alkyl chains. Lastly, a variety of secondary amines were employed in a β-formylation → reductive-amination strategy to produce amine-functionalized bacteriochlorins 18a-18e. The resulting amines were amenable to purification by silica gel column chromatography (EtOAc or CH2Cl2/MeOH/NH4OH as eluents). Subsequent N-alkylation of the amines was achieved using standard conditions, and the water-soluble cationic products that precipitated from the CHCl3 reaction mixtures were isolated by precipitation and centrifugation. Some of these compounds were investigated for their efficacy as antimicrobial photosensitizers [64]. Scheme 6. β-Substituted cationic ammonium bacteriochlorin derivatives prepared by Suzuki coupling, as described by the group of Lindsey [65].
Related compounds with terminal amine functional groups, such as 3,13-diaryl bacteriochlorin 22, were prepared using similar Suzuki coupling strategies. Bioconjugatable derivatives of these compounds carrying an NHS-ester functional group, such as 23, were also prepared by a regio-selective meso-bromination → Suzuki coupling sequence (see also Section 2.2.2) [65].
The group of Lindsey also prepared a range of amphiphilic bacteriochlorins of limited aqueous solubility bearing one amine side chain by reductive amination of a β-formylated bacteriochlorin (see also Scheme 5) [66]. A representative example is bacteriochlorin 24, which possesses an ammonium-terminated dialkyl chain, a so-called swallowtail functionality. This moiety was designed to project solubilizing groups above and below the plane of the macrocycle, leading to facial encumbrance that inhibits macrocycle stacking and increases hydrophilicity. A similar strategy was used to solubilize meso-aryl porphyrins in organic solvents [67,68].
Other ammonium-based water-soluble derivatives were also prepared by the Lindsey group by introduction of spiro-linked piperidine moieties at the β-positions of a bacteriochlorin [69]. The integral spiropiperidine functional groups were quarternized using standard conditions to furnish water-soluble derivatives, such as bacteriochlorin 25 (Figure 1). product 20 were removed, and the free amine quarternized by treatment with CH3I to afford the final ammonium-functionalized bacteriochlorin product 21. Scheme 6. β-Substituted cationic ammonium bacteriochlorin derivatives prepared by Suzuki coupling, as described by the group of Lindsey [65].
Related compounds with terminal amine functional groups, such as 3,13-diaryl bacteriochlorin 22, were prepared using similar Suzuki coupling strategies. Bioconjugatable derivatives of these compounds carrying an NHS-ester functional group, such as 23, were also prepared by a regioselective meso-bromination → Suzuki coupling sequence (see also Section 2.2.2) [65].
The group of Lindsey also prepared a range of amphiphilic bacteriochlorins of limited aqueous solubility bearing one amine side chain by reductive amination of a β-formylated bacteriochlorin (see also Scheme 5) [66]. A representative example is bacteriochlorin 24, which possesses an ammoniumterminated dialkyl chain, a so-called swallowtail functionality. This moiety was designed to project solubilizing groups above and below the plane of the macrocycle, leading to facial encumbrance that inhibits macrocycle stacking and increases hydrophilicity. A similar strategy was used to solubilize meso-aryl porphyrins in organic solvents [67,68].  The direct introduction of ammonium groups using a nucleophilic Senge arylation strategy was performed by Anderson and co-workers on 1,15 diaryl porphyrin 26Zn (Scheme 7) [70]. Porphyrin 26 was functionalized at the meso-position with a Boc-protected amino-phenyl group. The resulting derivative 27 was carried through multiple steps to afford porphyrin dimer 28 that was rendered water-soluble by quarternization of the amine functionality with CH 3 I. Other ammonium-based water-soluble derivatives were also prepared by the Lindsey group by introduction of spiro-linked piperidine moieties at the β-positions of a bacteriochlorin [69]. The integral spiropiperidine functional groups were quarternized using standard conditions to furnish watersoluble derivatives, such as bacteriochlorin 25 (Figure 1).
The direct introduction of ammonium groups using a nucleophilic Senge arylation strategy was performed by Anderson and co-workers on 1,15 diaryl porphyrin 26Zn (Scheme 7) [70]. Porphyrin 26 was functionalized at the meso-position with a Boc-protected amino-phenyl group. The resulting derivative 27 was carried through multiple steps to afford porphyrin dimer 28 that was rendered water-soluble by quarternization of the amine functionality with CH3I. Scheme 7. meso-Aryl-ammonium bis-acetylene linked porphyrin dimers prepared via Senge arylation, as described by the Anderson group [70]. DIPEA = N,N-diisopropylethylamine.

meso-Tetrakispyridiniumporphyrins
meso-Tetrapyridylporphyrins and the corresponding meso-tetrakis(methylpyridinium)porphyrins are long known, and their intercalation into DNA was studied in detail [55,56]. Pyridinium porphyrins continue to attract attention as next generation photosensitizers for PDT. Various new mesotetrakispyridiniumporphyrin derivatives were prepared using a range of electrophiles to quarternize the pyridine nitrogens (Scheme 8).

Scheme 8. Quarternization options of meso-tetrakis(4-pyridyl)porphyrin.
Orlandi and co-workers prepared meso-tetrakis (4-pyridinium)porphyrins (31) by reaction of mesotetra(4-pyridyl)porphyrin (30) with various benzyl chlorides to study the effect of polar alkylating groups on their antibacterial activity [71]. The benzylation conditions required were more vigorous (reflux in  meso-Tetrapyridylporphyrins and the corresponding meso-tetrakis(methylpyridinium)-porphyrins are long known, and their intercalation into DNA was studied in detail [55,56]. Pyridinium porphyrins continue to attract attention as next generation photosensitizers for PDT. Various new meso-tetrakispyridiniumporphyrin derivatives were prepared using a range of electrophiles to quarternize the pyridine nitrogens (Scheme 8). Other ammonium-based water-soluble derivatives were also prepared by the Lindsey group by introduction of spiro-linked piperidine moieties at the β-positions of a bacteriochlorin [69]. The integral spiropiperidine functional groups were quarternized using standard conditions to furnish watersoluble derivatives, such as bacteriochlorin 25 (Figure 1).
The direct introduction of ammonium groups using a nucleophilic Senge arylation strategy was performed by Anderson and co-workers on 1,15 diaryl porphyrin 26Zn (Scheme 7) [70]. Porphyrin 26 was functionalized at the meso-position with a Boc-protected amino-phenyl group. The resulting derivative 27 was carried through multiple steps to afford porphyrin dimer 28 that was rendered water-soluble by quarternization of the amine functionality with CH3I. Scheme 7. meso-Aryl-ammonium bis-acetylene linked porphyrin dimers prepared via Senge arylation, as described by the Anderson group [70]. DIPEA = N,N-diisopropylethylamine.

meso-Tetrakispyridiniumporphyrins
meso-Tetrapyridylporphyrins and the corresponding meso-tetrakis(methylpyridinium)porphyrins are long known, and their intercalation into DNA was studied in detail [55,56]. Pyridinium porphyrins continue to attract attention as next generation photosensitizers for PDT. Various new mesotetrakispyridiniumporphyrin derivatives were prepared using a range of electrophiles to quarternize the pyridine nitrogens (Scheme 8).
Fluorinated derivatives of mor p-linked meso-pyridyl porphyrins were prepared along Adler synthesis routes [75]. N-Alkylation of the pyridyl substituents by treatment with (CH 3 ) 3 O + BF 4 − afforded the tetra-alkylated products 32 and 33, respectively, as their tetrafluoroborate salts ( Figure 2). DMF for 24 h) than typical for pyridine alkylations using alkyl halides. The water-soluble products were recovered by precipitation with Et2O and filtration. Similarly, Ghazaryan and co-workers prepared a variety of meso-substituted N-substituted tetrapyridiniumporphyrins with different central metals (Ag, Zn, Co and Fe) and alkylating agents (allyl-, oxyethyl-, butyl-and methallyl-substituted derivatives) [72]. A PEGylated derivative of meso-tetrakispyridiniumporphyrin was also prepared by alkylation of meso-tetra(4-pyridyl)-porphyrin with a short PEG-bromide [73,74]. Fluorinated derivatives of m-or p-linked meso-pyridyl porphyrins were prepared along Adler synthesis routes [75]. N-Alkylation of the pyridyl substituents by treatment with (CH3)3O + BF4 − afforded the tetra-alkylated products 32 and 33, respectively, as their tetrafluoroborate salts ( Figure 2). In search of dual-action photo-and cytotoxic anti-cancer agents, various metal complexes were coordinated to the outer pyridyl nitrogens in tetrapyridylporphyrins (Scheme 9). Ruthenium, rhodium and iridium complexes were thus prepared by Therrien and co-workers [76] by treatment of meso-tetrapyridylporphyrin 30 with various metal arene salts to afford the water-soluble organic metallic complexes of type 34. They also prepared mixed arene-ruthenium substituted porphyrins in a similar manner, producing mono-and tetrametallated derivatives of 3-and 4-tetrapyridylporphyrins [77]. Both cis-and trans-platin conjugates of porphyrins were prepared by treatment of 30 with cis-or trans-Pt(II) complexes, respectively [77]. The gallium complexes of these compounds (such as 35) were prepared by Odani and co-workers [78] and also tested as photosensitizers for cancer therapy. In addition, tetrapyridylporphyrins with ruthenium nitrosyl groups substituted at their periphery were reported by the group of Alessio, generated by reaction of 30 with ruthenium nitrosyls and purified by column chromatography (CHCl3/5% EtOH as eluent) [79].

A3B and Other meso-Pyridiniumporphyrins
A number of symmetrically substituted pyridylporphyrins have been prepared in the search for the next generation of anticancer PDT agents. However, to further optimize their tumor-targeting and biodistribution properties, the porphyrin needs to be amenable to further modifications that will allow, for example, the conjugation of the porphyrin to a targeting molecule. Thus, a variety of examples emerged that use A3B porphyrins bearing three meso-pyridinium groups as the watersoluble framework of the chromophore, with the fourth meso-aryl ring available for further manipulations (Scheme 10). The parent A3B porphyrins are typically synthesized as statistical mixtures by Adler condensation of pyridylaldehyde, the desired arylaldehydes, and pyrrole, followed by chromatographic separation of the product mixture. The A3B porphyrin precursors are functionalized at the remaining meso-aryl group and N-alkylated with CH3I, with the order of these operations depending on the functionality present (see below).
Using this strategy, a pyrene-substituted trispyridyl A3B porphyrin could be prepared [80] (Scheme 10). Its N-alkylation with methyl p-toluenesulfonate in refluxing CHCl3/CH3NO2 afforded the tris-N-methyl pyridiniumporphyrin 37b. The group of Boyle synthesized tripyridyl A3B porphyrin 37a with the fourth aryl ring bearing a bioconjugatable isocyanate group. In search of dual-action photo-and cytotoxic anti-cancer agents, various metal complexes were coordinated to the outer pyridyl nitrogens in tetrapyridylporphyrins (Scheme 9). Ruthenium, rhodium and iridium complexes were thus prepared by Therrien and co-workers [76] by treatment of meso-tetrapyridylporphyrin 30 with various metal arene salts to afford the water-soluble organic metallic complexes of type 34. They also prepared mixed arene-ruthenium substituted porphyrins in a similar manner, producing mono-and tetrametallated derivatives of 3-and 4-tetrapyridyl-porphyrins [77]. Both cisand trans-platin conjugates of porphyrins were prepared by treatment of 30 with cisor trans-Pt(II) complexes, respectively [77]. The gallium complexes of these compounds (such as 35) were prepared by Odani and co-workers [78] and also tested as photosensitizers for cancer therapy. In addition, tetrapyridylporphyrins with ruthenium nitrosyl groups substituted at their periphery were reported by the group of Alessio, generated by reaction of 30 with ruthenium nitrosyls and purified by column chromatography (CHCl 3 /5% EtOH as eluent) [79].

A 3 B and Other meso-Pyridiniumporphyrins
A number of symmetrically substituted pyridylporphyrins have been prepared in the search for the next generation of anticancer PDT agents. However, to further optimize their tumor-targeting and biodistribution properties, the porphyrin needs to be amenable to further modifications that will allow, for example, the conjugation of the porphyrin to a targeting molecule. Thus, a variety of examples emerged that use A 3 B porphyrins bearing three meso-pyridinium groups as the water-soluble framework of the chromophore, with the fourth meso-aryl ring available for further manipulations (Scheme 10). The parent A 3 B porphyrins are typically synthesized as statistical mixtures by Adler condensation of pyridylaldehyde, the desired arylaldehydes, and pyrrole, followed by chromatographic separation of the product mixture. The A 3 B porphyrin precursors are functionalized at the remaining meso-aryl group and N-alkylated with CH 3 I, with the order of these operations depending on the functionality present (see below).
The N-alkylation step (standard CH3I alkylation conditions) needed to be performed after the formation of the isocyanate group to avoid unwanted N-alkylation of the amine precursors [81]. A number of p-substituted phenyl derivatives allowed a wide range of functionalizations. For instance, Song et al. synthesized A3B pyridyl porphyrin 37j with the fourth aryl group bearing a Pt(II) complex linked to the hydroxyl group of the meso-phenol group by a triethylene glycol linker [82]. N-Alkylation of the three pyridyl groups, followed by Boc-deprotection and complexation with the Pt(II) precursor, yielded the A3B platinum-porphyrin conjugate 37j. A similar approach was taken by the group of Alessio to synthesize water-soluble 99m Tc(I)/Re(I)-porphyrin conjugates, such as 37l, utilizing an amide-linked spacer between the aryl group and the 99m Tc(I)/Re(I) ion [83,84]. The watersoluble derivatives were purified by normal phase silica gel column chromatography (CH2Cl2/MeOH mixtures). These types of compounds can also be conjugated to cancer-targeting peptides for use in cancer therapy [85]. Cu(II)-based acylhydrazone porphyrin-derivatives 37m and 37n could be obtained using a similar strategy [86]. The group of Boyle synthesized an A3B porphyrin that could be further functionalized to establish an azide group [87]. The azide functionality was used in a click reaction to introduce an 18 F-terminated short PEG chain to generate water-soluble porphyrin 37k for PDT/PET theranostic applications [87]. After N-methylation of the pyridyl nitrogens, the subsequent synthetic steps required precipitation of the product using Et2O/MeOH mixtures. The final products were purified by passing through a column of neutral alumina.
The N-alkylation step (standard CH 3 I alkylation conditions) needed to be performed after the formation of the isocyanate group to avoid unwanted N-alkylation of the amine precursors [81]. A number of p-substituted phenyl derivatives allowed a wide range of functionalizations. For instance, Song et al. synthesized A 3 B pyridyl porphyrin 37j with the fourth aryl group bearing a Pt(II) complex linked to the hydroxyl group of the meso-phenol group by a triethylene glycol linker [82]. N-Alkylation of the three pyridyl groups, followed by Boc-deprotection and complexation with the Pt(II) precursor, yielded the A 3 B platinum-porphyrin conjugate 37j. A similar approach was taken by the group of Alessio to synthesize water-soluble 99m Tc(I)/Re(I)-porphyrin conjugates, such as 37l, utilizing an amide-linked spacer between the aryl group and the 99m Tc(I)/Re(I) ion [83,84]. The water-soluble derivatives were purified by normal phase silica gel column chromatography (CH 2 Cl 2 /MeOH mixtures). These types of compounds can also be conjugated to cancer-targeting peptides for use in cancer therapy [85]. Cu(II)-based acylhydrazone porphyrin-derivatives 37m and 37n could be obtained using a similar strategy [86]. The group of Boyle synthesized an A 3 B porphyrin that could be further functionalized to establish an azide group [87]. The azide functionality was used in a click reaction to introduce an 18 F-terminated short PEG chain to generate water-soluble porphyrin 37k for PDT/PET theranostic applications [87]. After N-methylation of the pyridyl nitrogens, the subsequent synthetic steps required precipitation of the product using Et 2 O/MeOH mixtures. The final products were purified by passing through a column of neutral alumina.
Gasparyan and co-workers synthesized an A 3 B amphiphilic trispyridylporphyrin with one meso-aryl group carrying a long alkyl chain using a mixed aldehyde Adler condensation [88]. Quarternization of the pyridyl groups with 3-bromopropene provided the water-soluble vinyl-substituted trispyridiniumporphyrins 38 and 38Ag ( Figure 3) that were isolated by precipitation with acetone.  Yasuda and co-workers prepared AB3 phosphorus porphyrin 39 [89]. Its axial chloro-ligands could be exchanged for simple alcohols and oligoethylene glycol chains to generate hydrophilic phosphorus porphyrins 40 and 41. N-Alkylation of the meso-pyridyl group in 40a-40d or 41 then furnished water-soluble derivatives, with solubility in water of around ~10 mM for compounds 42a-42d and 43.
Using a fundamentally different strategy toward meso-pyridyl porphyrins, pyridyl substituents can be introduced to meso-brominated porphyrins by using Suzuki couplings. For instance, the group of Lindsey reported the synthesis of a series of amphiphilic hydroporphyrins prepared by Suzuki coupling of a pyridyl boronic ester with meso-bromo-chlorins or bacteriochlorins [34]. Key chlorin  Yasuda and co-workers prepared AB3 phosphorus porphyrin 39 [89]. Its axial chloro-ligands could be exchanged for simple alcohols and oligoethylene glycol chains to generate hydrophilic phosphorus porphyrins 40 and 41. N-Alkylation of the meso-pyridyl group in 40a-40d or 41 then furnished water-soluble derivatives, with solubility in water of around ~10 mM for compounds 42a-42d and 43.
Using a fundamentally different strategy toward meso-pyridyl porphyrins, pyridyl substituents can be introduced to meso-brominated porphyrins by using Suzuki couplings. For instance, the group of Lindsey reported the synthesis of a series of amphiphilic hydroporphyrins prepared by Suzuki coupling of a pyridyl boronic ester with meso-bromo-chlorins or bacteriochlorins [34]. Key chlorin Yasuda and co-workers prepared AB 3 phosphorus porphyrin 39 [89]. Its axial chloro-ligands could be exchanged for simple alcohols and oligoethylene glycol chains to generate hydrophilic phosphorus porphyrins 40 and 41. N-Alkylation of the meso-pyridyl group in 40a-40d or 41 then furnished water-soluble derivatives, with solubility in water of around~10 mM for compounds 42a-42d and 43. (Scheme 11) [89]. An equivalent methodology was used to introduce axial PEG chains [90].
Using a fundamentally different strategy toward meso-pyridyl porphyrins, pyridyl substituents can be introduced to meso-brominated porphyrins by using Suzuki couplings. For instance, the group of Lindsey reported the synthesis of a series of amphiphilic hydroporphyrins prepared by Suzuki coupling of a pyridyl boronic ester with meso-bromo-chlorins or bacteriochlorins [34]. Key chlorin building block 45 was prepared by regioselective meso-bromination of chlorin 44 using NBS (Scheme 12) [91]. In the final step of the synthesis, the pyridyl functional group was quarternized with CH 3 I to furnish bacteriochlorin 46. This strategy is flexible and tolerant of a number of other substituents on the hydroporphyrin framework. Thus, chlorin 47 and bacteriochlorin 48 were prepared along analogous routes. building block 45 was prepared by regioselective meso-bromination of chlorin 44 using NBS (Scheme 12) [91]. In the final step of the synthesis, the pyridyl functional group was quarternized with CH3I to furnish bacteriochlorin 46. This strategy is flexible and tolerant of a number of other substituents on the hydroporphyrin framework. Thus, chlorin 47 and bacteriochlorin 48 were prepared along analogous routes.
In an analogous manner, Anderson and co-workers employed a Suzuki coupling strategy to introduce pyridyl functional groups to meso-dibrominated bis-acetylene linked porphyrin dimer 49 (Scheme 13) [70]. After coupling with 4-pyridinylboronic acid, both meso-pyridyl functional groups in 50 were methylated under standard conditions to afford the dicationic product 51. This water-soluble porphyrin dimer was purified by precipitation from DMF/Et2O. Scheme 11. Water-soluble AB 3 phosphorus porphyrins, as described by the group of Yasuda [89]. building block 45 was prepared by regioselective meso-bromination of chlorin 44 using NBS (Scheme 12) [91]. In the final step of the synthesis, the pyridyl functional group was quarternized with CH3I to furnish bacteriochlorin 46. This strategy is flexible and tolerant of a number of other substituents on the hydroporphyrin framework. Thus, chlorin 47 and bacteriochlorin 48 were prepared along analogous routes.
In an analogous manner, Anderson and co-workers employed a Suzuki coupling strategy to introduce pyridyl functional groups to meso-dibrominated bis-acetylene linked porphyrin dimer 49 (Scheme 13) [70]. After coupling with 4-pyridinylboronic acid, both meso-pyridyl functional groups in 50 were methylated under standard conditions to afford the dicationic product 51. This water-soluble porphyrin dimer was purified by precipitation from DMF/Et2O.

Other Pyridyl-Substituted Porphyrins
Porphyrins bearing alkylated pyridinium substituents in positions not directly linked to the meso-or β-positions of the macrocycle were also prepared. For example, Marzilli and co-workers synthesized porphyrins 52 ( Figure 4) with the pyridyl groups linked through sulfonamide linkages to the p-phenyl positions of meso-tetraarylporphyrins [59,95]. They investigated whether distant pyridinium groups are equally competent in mediating DNA-intercalation. Dipicolylamine (DPA) substituents could also be linked through the sulfonamide group (53), to prepare rhenium-based radiopharmaceuticals [96]. A remarkable octapyridiniumporphyrin 55 was prepared by Prato and co-workers [97] by treatment of meso-tetrakis(2,6-bis-(bromomethyl)-4-t-butylphenyl) porphyrin 54 with t-butylpyridine (Scheme 14). The octapyridyl porphyrin 55 was purified by crystallization from Et2O/MeOH. The octacationic compound 55 was used in studies toward assemblies for light-harvesting applications. A remarkable octapyridiniumporphyrin 55 was prepared by Prato and co-workers [97] by treatment of meso-tetrakis(2,6-bis-(bromomethyl)-4-t-butylphenyl) porphyrin 54 with t-butylpyridine (Scheme 14). The octapyridyl porphyrin 55 was purified by crystallization from Et 2 O/MeOH. The octacationic compound 55 was used in studies toward assemblies for light-harvesting applications. The introduction of pyridinium groups can also be achieved by esterification of a β-alkylester with a suitable pyridine-derivatized alcohol. Thus, cationic water-soluble ester 56 was prepared from chlorin e6 (11) by esterification with 2-(2-hydroxyethyl)pyridine, followed by quarternization with CH3I (cf. Scheme 4) [62]. Derivatives 56 ( Figure 5) and related 13 possess sharp absorbance spectra in Tris-HCl buffer at pH 7.6, indicating little aggregation of the chromophores. Pyridinium substituents have also been introduced in the axial positions of phosphorus and antimony meso-tetraphenyl porphyrins by axial exchange using a pyridine-derivatized alcohol (cf. to Scheme 11) [89,98]. Alkylation of the axial pyridyl moiety with a range of alkyl bromides furnished derivatives such as 57 ( Figure 5), with a water-solubility of ~3 mM [89].

meso-Imidazolium Porphyrins
The synthesis of porphyrins carrying N-alkylated meso-imidazolyl functionalities represents another strategy for the preparation of cationic porphyrins [99]. Lindsey and co-workers prepared porphyrins with one or two meso-imidazolyl groups by starting from imidazole-functionalized dipyrromethane precursors [100,101]. Mono-imidazolyl porphyrin 58 was alkylated with various alkylating reagents. The resulting imidazolium porphyrins were studied for their use in photodynamic therapy. The zwitterionic imidazolium sulfonate porphyrin 60Zn, for example, is the product obtained when 1,4-butane sultone was used as the alkylating reagent (Scheme 15) [100]. Scheme 14. An octapyridiniumporphyrin, as described by the group of Prato [97].
The introduction of pyridinium groups can also be achieved by esterification of a β-alkylester with a suitable pyridine-derivatized alcohol. Thus, cationic water-soluble ester 56 was prepared from chlorin e6 (11) by esterification with 2-(2-hydroxyethyl)pyridine, followed by quarternization with CH 3 I (cf. Scheme 4) [62]. Derivatives 56 ( Figure 5) and related 13 possess sharp absorbance spectra in Tris-HCl buffer at pH 7.6, indicating little aggregation of the chromophores. The introduction of pyridinium groups can also be achieved by esterification of a β-alkylester with a suitable pyridine-derivatized alcohol. Thus, cationic water-soluble ester 56 was prepared from chlorin e6 (11) by esterification with 2-(2-hydroxyethyl)pyridine, followed by quarternization with CH3I (cf. Scheme 4) [62]. Derivatives 56 ( Figure 5) and related 13 possess sharp absorbance spectra in Tris-HCl buffer at pH 7.6, indicating little aggregation of the chromophores. Pyridinium substituents have also been introduced in the axial positions of phosphorus and antimony meso-tetraphenyl porphyrins by axial exchange using a pyridine-derivatized alcohol (cf. to Scheme 11) [89,98]. Alkylation of the axial pyridyl moiety with a range of alkyl bromides furnished derivatives such as 57 ( Figure 5), with a water-solubility of ~3 mM [89].

meso-Imidazolium Porphyrins
The synthesis of porphyrins carrying N-alkylated meso-imidazolyl functionalities represents another strategy for the preparation of cationic porphyrins [99]. Lindsey and co-workers prepared porphyrins with one or two meso-imidazolyl groups by starting from imidazole-functionalized dipyrromethane precursors [100,101]. Mono-imidazolyl porphyrin 58 was alkylated with various alkylating reagents. The resulting imidazolium porphyrins were studied for their use in photodynamic therapy. The zwitterionic imidazolium sulfonate porphyrin 60Zn, for example, is the product obtained when 1,4-butane sultone was used as the alkylating reagent (Scheme 15) [100]. Pyridinium substituents have also been introduced in the axial positions of phosphorus and antimony meso-tetraphenyl porphyrins by axial exchange using a pyridine-derivatized alcohol (cf. to Scheme 11) [89,98]. Alkylation of the axial pyridyl moiety with a range of alkyl bromides furnished derivatives such as 57 ( Figure 5), with a water-solubility of~3 mM [89].

meso-Imidazolium Porphyrins
The synthesis of porphyrins carrying N-alkylated meso-imidazolyl functionalities represents another strategy for the preparation of cationic porphyrins [99]. Lindsey and co-workers prepared porphyrins with one or two meso-imidazolyl groups by starting from imidazole-functionalized dipyrromethane precursors [100,101]. Mono-imidazolyl porphyrin 58 was alkylated with various alkylating reagents. The resulting imidazolium porphyrins were studied for their use in photodynamic therapy. The zwitterionic imidazolium sulfonate porphyrin 60Zn, for example, is the product obtained when 1,4-butane sultone was used as the alkylating reagent (Scheme 15) [100].

Porphyrins with Carboxylate Functional Groups
Many naturally occurring porphyrins contain acetic acid or propionic acid side chains [102]. With increasing number of acid side chains, their solubility in aqueous solution increases, with the uroporphyrins being freely soluble, particularly in solutions of basic pH (Scheme 16) [102]. This suggests that the introduction of carboxylic acid functional groups to the periphery of porphyrins might be an effective way of furnishing water-soluble derivatives. This is, in fact, also observed. To simplify the purification of the porphyrins, the carboxylate groups are often masked throughout the synthesis as esters and are revealed by saponification in the final step.
meso-Tetrakis(4-carboxyphenyl)porphyrin, and its ester, are well known, and readily synthesized by condensation of the corresponding aldehydes with pyrrole [103][104][105]. They are also commercially available [58]. Carboxylate groups may also be introduced to the porphyrin by starting with more elaborate building blocks containing esters. Classic carboxylated meso-aryl porphyrins, such as meso-tetrakis(4-carboxyphenyl)porphyrin, have been prepared by Adler synthesis with estersubstituted benzaldehydes followed by saponification of the esters [40]. Tetracarboxylated palladium porphyrin 62 was prepared thusly, whereby the carboxylate moieties were revealed by standard ester saponification conditions after the palladium insertion step (Scheme 17) [106].
An introduction of esters to the β-positions of a porphyrin from ester-substituted building blocks is also possible, as illustrated by the synthesis of carboxylated benzoporphyrins starting from an ester-functionalized isoindole (Scheme 18) [107]. A retro-Diels-Alder reaction of 63 with concomitant saponification of the methyl esters afforded octacarboxylate 64. Protonation provided the octaacid 65 that also precipitated under these conditions. The water-solubility of the sodium salt 64 was determined to be 0.111 M [107].

Porphyrins with Carboxylate Functional Groups
Many naturally occurring porphyrins contain acetic acid or propionic acid side chains [102]. With increasing number of acid side chains, their solubility in aqueous solution increases, with the uroporphyrins being freely soluble, particularly in solutions of basic pH (Scheme 16) [102].

Porphyrins with Carboxylate Functional Groups
Many naturally occurring porphyrins contain acetic acid or propionic acid side chains [102]. With increasing number of acid side chains, their solubility in aqueous solution increases, with the uroporphyrins being freely soluble, particularly in solutions of basic pH (Scheme 16) [102]. This suggests that the introduction of carboxylic acid functional groups to the periphery of porphyrins might be an effective way of furnishing water-soluble derivatives. This is, in fact, also observed. To simplify the purification of the porphyrins, the carboxylate groups are often masked throughout the synthesis as esters and are revealed by saponification in the final step.
meso-Tetrakis(4-carboxyphenyl)porphyrin, and its ester, are well known, and readily synthesized by condensation of the corresponding aldehydes with pyrrole [103][104][105]. They are also commercially available [58]. Carboxylate groups may also be introduced to the porphyrin by starting with more elaborate building blocks containing esters. Classic carboxylated meso-aryl porphyrins, such as meso-tetrakis(4-carboxyphenyl)porphyrin, have been prepared by Adler synthesis with estersubstituted benzaldehydes followed by saponification of the esters [40]. Tetracarboxylated palladium porphyrin 62 was prepared thusly, whereby the carboxylate moieties were revealed by standard ester saponification conditions after the palladium insertion step (Scheme 17) [106].
An introduction of esters to the β-positions of a porphyrin from ester-substituted building blocks is also possible, as illustrated by the synthesis of carboxylated benzoporphyrins starting from an ester-functionalized isoindole (Scheme 18) [107]. A retro-Diels-Alder reaction of 63 with concomitant saponification of the methyl esters afforded octacarboxylate 64. Protonation provided the octaacid 65 that also precipitated under these conditions. The water-solubility of the sodium salt 64 was determined to be 0.111 M [107]. This suggests that the introduction of carboxylic acid functional groups to the periphery of porphyrins might be an effective way of furnishing water-soluble derivatives. This is, in fact, also observed. To simplify the purification of the porphyrins, the carboxylate groups are often masked throughout the synthesis as esters and are revealed by saponification in the final step.
meso-Tetrakis(4-carboxyphenyl)porphyrin, and its ester, are well known, and readily synthe-sized by condensation of the corresponding aldehydes with pyrrole [103][104][105]. They are also commercially available [58]. Carboxylate groups may also be introduced to the porphyrin by starting with more elaborate building blocks containing esters. Classic carboxylated meso-aryl porphyrins, such as meso-tetrakis(4-carboxyphenyl)porphyrin, have been prepared by Adler synthesis with ester-substituted benzaldehydes followed by saponification of the esters [40]. Tetracarboxylated palladium porphyrin 62 was prepared thusly, whereby the carboxylate moieties were revealed by standard ester saponification conditions after the palladium insertion step (Scheme 17) [106].
An introduction of esters to the β-positions of a porphyrin from ester-substituted building blocks is also possible, as illustrated by the synthesis of carboxylated benzoporphyrins starting from an ester-functionalized isoindole (Scheme 18) [107]. A retro-Diels-Alder reaction of 63 with concomitant saponification of the methyl esters afforded octacarboxylate 64. Protonation provided the octaacid 65 that also precipitated under these conditions. The water-solubility of the sodium salt 64 was determined to be 0.111 M [107]. Water-soluble acetylene-linked bis(imidazolylporphyrins) were prepared from starting materials bearing protected acid functionalities. Thus, ester-functionalized aldehyde and dipyrromethane were Scheme 17. Carboxylated meso-aryl porphyrins, as described by the group of Skondra [106]. Water-soluble acetylene-linked bis(imidazolylporphyrins) were prepared from starting materials bearing protected acid functionalities. Thus, ester-functionalized aldehyde and dipyrromethane were Scheme 18. Carboxylated benzoporphyrins, as described by the group of Sugimoto [107]. Water-soluble acetylene-linked bis(imidazolylporphyrins) were prepared from starting materials bearing protected acid functionalities. Thus, ester-functionalized aldehyde and dipyrromethane were Scheme 19. Porphyrin dimers and trimers bearing carboxylate groups in the meso-positions, as described by the group of Kobuke [108,109].
Water-soluble acetylene-linked bis(imidazolylporphyrins) were prepared from starting materials bearing protected acid functionalities. Thus, ester-functionalized aldehyde and dipyrromethane were condensed and oxidized to synthesize porphyrin 66 bearing ester-terminated alkyl chains in the meso-positions. The ester moieties were carried through the entire synthesis of the porphyrin dimer and the carboxylates were only deprotected in the last step (Scheme 19) [108]. Using this strategy, bulky bis(carboxylethyl)methyl substituents could also be introduced to the meso-positions early in the synthesis to furnish dimers of type 68 and trimers of type 69, which showed less aggregation in water [109].
Lindsey and co-workers prepared carboxylated trans-AB porphyrins using a 2 + 2 dipyrromethane condensation strategy, using dipyrromethane 70 carrying a protected 2,4,6-triester-subsituted meso-phenyl group (Scheme 20) [110]. The condensation of 70 and counterpart 71 in the presence of zinc afforded the zinc-porphyrin triester 72, which could be saponified to afford the tricarboxylic acid 73a. Along an analogous route, trans-AB porphyrins 73b and 73c bearing bioconjugatable groups at the meso-position opposite the solubilizing groups were prepared. condensed and oxidized to synthesize porphyrin 66 bearing ester-terminated alkyl chains in the meso-positions. The ester moieties were carried through the entire synthesis of the porphyrin dimer and the carboxylates were only deprotected in the last step (Scheme 19) [108]. Using this strategy, bulky bis(carboxylethyl)methyl substituents could also be introduced to the meso-positions early in the synthesis to furnish dimers of type 68 and trimers of type 69, which showed less aggregation in water [109]. Lindsey and co-workers prepared carboxylated trans-AB porphyrins using a 2 + 2 dipyrromethane condensation strategy, using dipyrromethane 70 carrying a protected 2,4,6-triester-subsituted mesophenyl group (Scheme 20) [110]. The condensation of 70 and counterpart 71 in the presence of zinc afforded the zinc-porphyrin triester 72, which could be saponified to afford the tricarboxylic acid 73a. Along an analogous route, trans-AB porphyrins 73b and 73c bearing bioconjugatable groups at the meso-position opposite the solubilizing groups were prepared. Scheme 20. Carboxylated trans-AB porphyrins, as described by the group of Lindsey [110].
To maximize the number of carboxylic acid groups introduced, carboxylic acid ester-terminated dendritic components can be utilized, often bound to the porphyrin through amide linkages. For instance, treatment of tetrarylporphyrin acid chloride 74 with dimethyl iminodiacetate or its second generation dendrimer analogue, followed by saponification of the esters, afforded the polyacid porphyrins 75a or 75b, respectively (Scheme 21) [111]. They were purified by precipitation and filtration.
meso-Tetrakis(4-hydroxyphenyl)porphyrin (76) is a versatile starting material for the synthesis of hydrophilic derivatives since the p-phenolic oxygens can react with a variety of solubilizing groups. A4-Porphyrin 76 is synthesized through the Adler procedure, generally as its 4-methoxy derivative, that can be purified and handled easily. It is subsequently deprotected using BBr3 [14] (see also below, Schemes 23 and 47).
Using tetraphenol 76, Chen and co-workers also synthesized porphyrins bearing dendritic carboxylate groups, albeit their synthesis was less convergent than that of Mukhtar and co-workers [114], since the dendrimer generations were built up on the porphyrin core. Thus, 76 was converted to polyamine-derivatized porphyrin 77 in three steps. Reaction of the amines in 77 with bromoacetic Scheme 20. Carboxylated trans-AB porphyrins, as described by the group of Lindsey [110].
To maximize the number of carboxylic acid groups introduced, carboxylic acid ester-terminated dendritic components can be utilized, often bound to the porphyrin through amide linkages. For instance, treatment of tetrarylporphyrin acid chloride 74 with dimethyl iminodiacetate or its second generation dendrimer analogue, followed by saponification of the esters, afforded the polyacid porphyrins 75a or 75b, respectively (Scheme 21) [111]. They were purified by precipitation and filtration.
meso-Tetrakis(4-hydroxyphenyl)porphyrin (76) is a versatile starting material for the synthesis of hydrophilic derivatives since the p-phenolic oxygens can react with a variety of solubilizing groups. A 4 -Porphyrin 76 is synthesized through the Adler procedure, generally as its 4-methoxy derivative, that can be purified and handled easily. It is subsequently deprotected using BBr 3 [14] (see also below, Schemes 23 and 47).
Using tetraphenol 76, Chen and co-workers also synthesized porphyrins bearing dendritic carboxylate groups, albeit their synthesis was less convergent than that of Mukhtar and co-workers [114], since the dendrimer generations were built up on the porphyrin core. Thus, 76 was converted to polyamine-derivatized porphyrin 77 in three steps. Reaction of the amines in 77 with bromoacetic acid ethyl ester provided the protected porphyrin 78, followed by hydrolysis with TFA to give the free acid 79 (Scheme 22) [114]  Alkylation strategies have also been employed for the introduction of carboxylates. For instance, various carboxylated core-modified porphyrins were prepared by O-alkylation of the phenolic oxygens of a meso-4-hydroxyphenyl-substituted core-modified dithiaporphyrin. Like their aza-analogues, the requisite core-modified porphyrins were synthesized with a methyl-ether protecting group in the p-position of one or more phenyl groups and deprotected using the standard BBr 3 method. The phenolic oxygens were then alkylated with ethyl bromoacetate. Saponification of the installed esters furnished the dithiaporphyrin 81 bearing carboxylic acid functional groups (Scheme 23) [115]. Alkylation strategies have also been employed for the introduction of carboxylates. For instance, various carboxylated core-modified porphyrins were prepared by O-alkylation of the phenolic oxygens of a meso-4-hydroxyphenyl-substituted core-modified dithiaporphyrin. Like their aza-analogues, the requisite core-modified porphyrins were synthesized with a methyl-ether protecting group in the p-position of one or more phenyl groups and deprotected using the standard BBr3 method. The phenolic oxygens were then alkylated with ethyl bromoacetate. Saponification of the installed esters furnished the dithiaporphyrin 81 bearing carboxylic acid functional groups (Scheme 23) [115]. Scheme 23. Core-modified carboxylated porphyrin, as described by the group of Detty [115]. Diethylenetriamine-N,N,N′′,N′′-tetraacetate (DTTA) groups were also introduced to meso positions of a porphyrin by alkylation of meso-tetrakis(bromomethylphenyl)porphyrin [116]. The DTTA groups were introduced as protected t-butyl esters and deprotected using standard conditions. The water-soluble products were purified by sequential cation and anion exchange chromatography.
Prato and co-workers also used an alkylation strategy to synthesize octacarboxylated porphyrin 84, starting from a tetra(bromomethyl)-substituted porphyrin. Alkylation of porphyrin 82 with diethyl malonate afforded the tetramalonic ester-derivatized porphyrin 83, which was saponified to free the eight carboxylate moieties (Scheme 24) [97]. Octacarboxylate 84 precipitated under the saponification conditions and was isolated by filtration to afford the pure product. Carboxyphenyl substituents can also be directly introduced to the meso-positions of synthetic chlorins and bacteriochlorins by Suzuki coupling of suitable meso-bromo-substituted porphyrins with boronic esters derived from benzoic acid. Using the same Suzuki coupling approach that was used to introduce pyridyl substituents to the meso-position (cf. Scheme 12), chlorins 85, 86 and the bacteriochlorin 87 ( Figure 6) were prepared [91]. The carboxylate functionality was introduced in the free acid form, eliminating the need for the utilization of protecting groups. Scheme 23. Core-modified carboxylated porphyrin, as described by the group of Detty [115]. Diethylenetriamine-N,N,N ,N -tetraacetate (DTTA) groups were also introduced to meso positions of a porphyrin by alkylation of meso-tetrakis(bromomethylphenyl)porphyrin [116]. The DTTA groups were introduced as protected t-butyl esters and deprotected using standard conditions. The water-soluble products were purified by sequential cation and anion exchange chromatography.
Prato and co-workers also used an alkylation strategy to synthesize octacarboxylated porphyrin 84, starting from a tetra(bromomethyl)-substituted porphyrin. Alkylation of porphyrin 82 with diethyl malonate afforded the tetramalonic ester-derivatized porphyrin 83, which was saponified to free the eight carboxylate moieties (Scheme 24) [97]. Octacarboxylate 84 precipitated under the saponification conditions and was isolated by filtration to afford the pure product. Alkylation strategies have also been employed for the introduction of carboxylates. For instance, various carboxylated core-modified porphyrins were prepared by O-alkylation of the phenolic oxygens of a meso-4-hydroxyphenyl-substituted core-modified dithiaporphyrin. Like their aza-analogues, the requisite core-modified porphyrins were synthesized with a methyl-ether protecting group in the p-position of one or more phenyl groups and deprotected using the standard BBr3 method. The phenolic oxygens were then alkylated with ethyl bromoacetate. Saponification of the installed esters furnished the dithiaporphyrin 81 bearing carboxylic acid functional groups (Scheme 23) [115]. Scheme 23. Core-modified carboxylated porphyrin, as described by the group of Detty [115]. Diethylenetriamine-N,N,N′′,N′′-tetraacetate (DTTA) groups were also introduced to meso positions of a porphyrin by alkylation of meso-tetrakis(bromomethylphenyl)porphyrin [116]. The DTTA groups were introduced as protected t-butyl esters and deprotected using standard conditions. The water-soluble products were purified by sequential cation and anion exchange chromatography.
Prato and co-workers also used an alkylation strategy to synthesize octacarboxylated porphyrin 84, starting from a tetra(bromomethyl)-substituted porphyrin. Alkylation of porphyrin 82 with diethyl malonate afforded the tetramalonic ester-derivatized porphyrin 83, which was saponified to free the eight carboxylate moieties (Scheme 24) [97]. Octacarboxylate 84 precipitated under the saponification conditions and was isolated by filtration to afford the pure product. Carboxyphenyl substituents can also be directly introduced to the meso-positions of synthetic chlorins and bacteriochlorins by Suzuki coupling of suitable meso-bromo-substituted porphyrins with boronic esters derived from benzoic acid. Using the same Suzuki coupling approach that was used to introduce pyridyl substituents to the meso-position (cf. Scheme 12), chlorins 85, 86 and the bacteriochlorin 87 ( Figure 6) were prepared [91]. The carboxylate functionality was introduced in the free acid form, eliminating the need for the utilization of protecting groups. Carboxyphenyl substituents can also be directly introduced to the meso-positions of synthetic chlorins and bacteriochlorins by Suzuki coupling of suitable meso-bromo-substituted porphyrins with boronic esters derived from benzoic acid. Using the same Suzuki coupling approach that was used to introduce pyridyl substituents to the meso-position (cf. Scheme 12), chlorins 85, 86 and the bacteriochlorin 87 ( Figure 6) were prepared [91]. The carboxylate functionality was introduced in the free acid form, eliminating the need for the utilization of protecting groups.
As well starting from meso-brominated precursors, the group of Anderson used a Sonogashira coupling strategy to functionalize the meso-positions of a PEGylated porphyrin dimer with carboxylate groups. meso-Dibromoporphyrin dimer 49 was coupled with 5-ethynyl-1,3-benzenedicarboxylic acid to form the tetracarboxylated water-soluble porphyrin dimer 88 (Scheme 25) [70]. Again, it is noteworthy that the acid functionality was introduced in unprotected form. As well starting from meso-brominated precursors, the group of Anderson used a Sonogashira coupling strategy to functionalize the meso-positions of a PEGylated porphyrin dimer with carboxylate groups. meso-Dibromoporphyrin dimer 49 was coupled with 5-ethynyl-1,3-benzenedicarboxylic acid to form the tetracarboxylated water-soluble porphyrin dimer 88 (Scheme 25) [70]. Again, it is noteworthy that the acid functionality was introduced in unprotected form. Scheme 25. Carboxylated bis-acetylene linked porphyrin dimers, as described by the group of Anderson [70]. dba = dibenzylacetone. Scheme 26. Tetracarboxybacteriochlorins, as described by the group of Lindsey [117].
Functionalization of the β-position of bacteriochlorins with carboxyphenyl groups was also achieved by Suzuki coupling, albeit this method required the use of protected boronic ester carboxylates [117]. Thus, β-dibromoporphyrin 89 was functionalized using the boronic ester of the As well starting from meso-brominated precursors, the group of Anderson used a Sonogashira coupling strategy to functionalize the meso-positions of a PEGylated porphyrin dimer with carboxylate groups. meso-Dibromoporphyrin dimer 49 was coupled with 5-ethynyl-1,3-benzenedicarboxylic acid to form the tetracarboxylated water-soluble porphyrin dimer 88 (Scheme 25) [70]. Again, it is noteworthy that the acid functionality was introduced in unprotected form. Scheme 25. Carboxylated bis-acetylene linked porphyrin dimers, as described by the group of Anderson [70]. dba = dibenzylacetone. Scheme 26. Tetracarboxybacteriochlorins, as described by the group of Lindsey [117].
Functionalization of the β-position of bacteriochlorins with carboxyphenyl groups was also achieved by Suzuki coupling, albeit this method required the use of protected boronic ester carboxylates [117]. Thus, β-dibromoporphyrin 89 was functionalized using the boronic ester of the  Functionalization of the β-position of bacteriochlorins with carboxyphenyl groups was also achieved by Suzuki coupling, albeit this method required the use of protected boronic ester carboxylates [117]. Thus, β-dibromoporphyrin 89 was functionalized using the boronic ester of the t-butyl ester-protected 3,5-carboxyphenyl substituents (Scheme 26). The protecting groups were removed at the last step of the synthesis by acid treatment. Furthermore, the option for bioconjugation was demonstrated in these systems by Suzuki coupling of a meso-bromobacteriochlorin, generated by regioselective bromination of the parent bacteriochlorin, to produce hydrophilic tetracarboxyl-bacteriochlorin 94 [117]. As well starting from meso-brominated precursors, the group of Anderson used a Sonogashira coupling strategy to functionalize the meso-positions of a PEGylated porphyrin dimer with carboxylate groups. meso-Dibromoporphyrin dimer 49 was coupled with 5-ethynyl-1,3-benzenedicarboxylic acid to form the tetracarboxylated water-soluble porphyrin dimer 88 (Scheme 25) [70]. Again, it is noteworthy that the acid functionality was introduced in unprotected form. Scheme 25. Carboxylated bis-acetylene linked porphyrin dimers, as described by the group of Anderson [70]. dba = dibenzylacetone.
Functionalization of the β-position of bacteriochlorins with carboxyphenyl groups was also achieved by Suzuki coupling, albeit this method required the use of protected boronic ester carboxylates [117]. Thus, β-dibromoporphyrin 89 was functionalized using the boronic ester of the

Sulfonated Porphyrins
Sulfonation of meso-tetraphenylporphyrin proceeds regioselectively at the para-positions of the meso-phenyl rings [118]. This reaction led to the earliest examples of water-soluble meso-tetraaryl-porphyrins [40]. A number of sulfonated A 4 porphyrins were prepared by direct sulfonation methods [40], and are commercially available [58]. However, this solubilization strategy has drawbacks, not the least of which are the harsh reaction conditions (conc. H 2 SO 4 , ∆) required for the sulfonation step, and the difficulty in purifying the target compound. On the other hand, sulfonation readily leads to the solubilization of porphyrins in aqueous media. Interestingly, the porphyrin is protonated during the sulfonation step and is thus protected by the dicationic charge from getting sulfonated at the β-positions along an electrophilic aromatic substitution pathway, in contrast with the regioselective β-sulfonation of the less basic corroles using chlorosulfonic acid [119][120][121].
One particular challenge faced by using sulfonation procedures is the incorporation of other functional groups since they may be incompatible with the harsh sulfonation conditions. The sulfonation step is often employed directly after porphyrin formation, then subsequent modification of the porphyrin is performed. The drawback of this strategy is the difficulty in handling and purification of the sulfonated porphyrins.
Despite these disadvantages, the traditional direct sulfonation method was employed by Pillai and co-workers to regioselectively introduce sulfonate groups to the meso-p-phenyl positions of N-confused porphyrins (Scheme 27) [122]. Sulfonation of N-confused porphyrin 95 by treatment with H 2 SO 4 at elevated temperature over several hours afforded the tetrasulfonated porphyrin 96 that was tested as a photosensitizer for PDT [122]. The product was purified by precipitation and continuous Soxhlet extraction with MeOH. No further functionalizations of this porphyrin derivative were reported. t-butyl ester-protected 3,5-carboxyphenyl substituents (Scheme 26). The protecting groups were removed at the last step of the synthesis by acid treatment. Furthermore, the option for bioconjugation was demonstrated in these systems by Suzuki coupling of a meso-bromobacteriochlorin, generated by regioselective bromination of the parent bacteriochlorin, to produce hydrophilic tetracarboxylbacteriochlorin 94 [117].

Sulfonated Porphyrins
Sulfonation of meso-tetraphenylporphyrin proceeds regioselectively at the para-positions of the meso-phenyl rings [118]. This reaction led to the earliest examples of water-soluble meso-tetraarylporphyrins [40]. A number of sulfonated A4 porphyrins were prepared by direct sulfonation methods [40], and are commercially available [58]. However, this solubilization strategy has drawbacks, not the least of which are the harsh reaction conditions (conc. H2SO4, ∆) required for the sulfonation step, and the difficulty in purifying the target compound. On the other hand, sulfonation readily leads to the solubilization of porphyrins in aqueous media. Interestingly, the porphyrin is protonated during the sulfonation step and is thus protected by the dicationic charge from getting sulfonated at the β-positions along an electrophilic aromatic substitution pathway, in contrast with the regioselective β-sulfonation of the less basic corroles using chlorosulfonic acid [119][120][121].
One particular challenge faced by using sulfonation procedures is the incorporation of other functional groups since they may be incompatible with the harsh sulfonation conditions. The sulfonation step is often employed directly after porphyrin formation, then subsequent modification of the porphyrin is performed. The drawback of this strategy is the difficulty in handling and purification of the sulfonated porphyrins.
Despite these disadvantages, the traditional direct sulfonation method was employed by Pillai and co-workers to regioselectively introduce sulfonate groups to the meso-p-phenyl positions of N-confused porphyrins (Scheme 27) [122]. Sulfonation of N-confused porphyrin 95 by treatment with H2SO4 at elevated temperature over several hours afforded the tetrasulfonated porphyrin 96 that was tested as a photosensitizer for PDT [122]. The product was purified by precipitation and continuous Soxhlet extraction with MeOH. No further functionalizations of this porphyrin derivative were reported. Scheme 27. Sulfonated N-confused porphyrin, as described by the group of Pillai [122].
Likewise, asymmetric meso-aryl porphyrins were also subjected to sulfonation reactions. For instance, A3B porphyrin meso-trisphenyl-4-pyridylporphyrin, made by mixed aldehyde condensation, could be trisulfonated using oleum at 80 °C [123]. The pure product was obtained by precipitation and centrifugation after neutralization of the acid. The pyridyl moiety could then be functionalized with a platinum complex for study as a tumor targeting photosensitizer. The group of Lippard prepared the A3B porphyrin meso-trisphenyl-(2,6-nitrophenyl)porphyrin 97 (Scheme 28). Reduction of the nitro group afforded the 2,6-diaminophenyl porphyrin 98 that was subjected to sulfonation. The water-soluble product 99 was purified and isolated by reverse phase chromatography (RP-18). The purified free amine could then be functionalized with DPA for its use as a Zn 2+ chemosensor [124]. Furthermore, the manganese complex of 100 was prepared and used as a dual function contrast agent for the fluorescence imaging of Zn 2 and MRI in biological contexts [124]. Scheme 27. Sulfonated N-confused porphyrin, as described by the group of Pillai [122].
Likewise, asymmetric meso-aryl porphyrins were also subjected to sulfonation reactions. For instance, A 3 B porphyrin meso-trisphenyl-4-pyridylporphyrin, made by mixed aldehyde condensation, could be trisulfonated using oleum at 80 • C [123]. The pure product was obtained by precipitation and centrifugation after neutralization of the acid. The pyridyl moiety could then be functionalized with a platinum complex for study as a tumor targeting photosensitizer. The group of Lippard prepared the A 3 B porphyrin meso-trisphenyl-(2,6-nitrophenyl)porphyrin 97 (Scheme 28). Reduction of the nitro group afforded the 2,6-diaminophenyl porphyrin 98 that was subjected to sulfonation. The water-soluble product 99 was purified and isolated by reverse phase chromatography (RP-18). The purified free amine could then be functionalized with DPA for its use as a Zn 2+ chemosensor [124]. Furthermore, the manganese complex of 100 was prepared and used as a dual function contrast agent for the fluorescence imaging of Zn 2 and MRI in biological contexts [124].
As the previous examples have shown, some functionalities tolerate the sulfonation conditions. Surprisingly, this is also the case for isoindoline nitroxide-functionalized A 3 B porphyrin 101. All phenyl substituents could be sulfonated by treatment with H 2 SO 4 with retention of the isoindoline nitroxide (Scheme 29), albeit the yield for the water-soluble final product 102 was low (~30%) [125]. As the previous examples have shown, some functionalities tolerate the sulfonation conditions. Surprisingly, this is also the case for isoindoline nitroxide-functionalized A3B porphyrin 101. All phenyl substituents could be sulfonated by treatment with H2SO4 with retention of the isoindoline nitroxide (Scheme 29), albeit the yield for the water-soluble final product 102 was low (~30%) [125]. Scheme 29. Sulfonated isoindoline nitroxide-functionalized A3B porphyrin, as described by the group of Yang [125].
A chlorosulfonation method has been used for the introduction of sulfonic acid groups to a number of halogenated meso-aryl porphyrins by the group of Wyatt and co-workers (Scheme 30) [126]. Treatment of chlorinated porphyrin 103, for example, with chlorosulfonic acid afforded chlorosulfonation product 104 that was hydrolyzed by suspension in H2O to provide the corresponding sulfonic acid product 105. Alternatively, the chlorosulfonate could also be converted to sulfonamide derivatives by reaction with amines [126]. The corresponding chlorin and bacteriochlorin 106 and 107, respectively, were made by diimide reduction of the sulfonated porphyrin 105, and were tested as photosensitizers for the PDT of tumors (Scheme 30) [127]. Scheme 28. Sulfonated A 3 B porphyrin bearing DPA substituents for fluorescence sensing of Zn 2+ , as described by the group of Lippard [124]. As the previous examples have shown, some functionalities tolerate the sulfonation conditions. Surprisingly, this is also the case for isoindoline nitroxide-functionalized A3B porphyrin 101. All phenyl substituents could be sulfonated by treatment with H2SO4 with retention of the isoindoline nitroxide (Scheme 29), albeit the yield for the water-soluble final product 102 was low (~30%) [125]. Scheme 29. Sulfonated isoindoline nitroxide-functionalized A3B porphyrin, as described by the group of Yang [125].
A chlorosulfonation method has been used for the introduction of sulfonic acid groups to a number of halogenated meso-aryl porphyrins by the group of Wyatt and co-workers (Scheme 30) [126]. Treatment of chlorinated porphyrin 103, for example, with chlorosulfonic acid afforded chlorosulfonation product 104 that was hydrolyzed by suspension in H2O to provide the corresponding sulfonic acid product 105. Alternatively, the chlorosulfonate could also be converted to sulfonamide derivatives by reaction with amines [126]. The corresponding chlorin and bacteriochlorin 106 and 107, respectively, were made by diimide reduction of the sulfonated porphyrin 105, and were tested as photosensitizers for the PDT of tumors (Scheme 30) [127]. Scheme 29. Sulfonated isoindoline nitroxide-functionalized A 3 B porphyrin, as described by the group of Yang [125].
A chlorosulfonation method has been used for the introduction of sulfonic acid groups to a number of halogenated meso-aryl porphyrins by the group of Wyatt and co-workers (Scheme 30) [126]. Treatment of chlorinated porphyrin 103, for example, with chlorosulfonic acid afforded chlorosulfonation product 104 that was hydrolyzed by suspension in H 2 O to provide the corresponding sulfonic acid product 105. Alternatively, the chlorosulfonate could also be converted to sulfonamide derivatives by reaction with amines [126]. The corresponding chlorin and bacteriochlorin 106 and 107, respectively, were made by diimide reduction of the sulfonated porphyrin 105, and were tested as photosensitizers for the PDT of tumors (Scheme 30) [127].
The attachment of sulfonated groups to the β-positions of a tetrapyrrolic macrocycle is an alternative method toward the generation of hydrophilic sulfonated derivatives. This approach was applied to the generation of alkylsulfonated bacteriochlorins [128]. For example, sulfonated bacterio-chlorophyll derivatives were prepared by reaction of Pd-bacteriopheophorbide (108) with homo-taurine (Scheme 31) [128]. Treatment of either 109 or the sulfo-NHS ester 110 with a second equivalent of homotaurine also yielded the bis-sulfonated product 111 (with the trisulfonated compound arising from imine formation with the β-acetyl group as a minor product). Bacteriochlorin 112M could also prepared using a similar procedure using taurine as the nucleophile. All of the sulfonated derivatives were found to possess high solubility in water (up to 40 mg/mL) [129].
The products were either purified by HPLC (MeOH/phosphate-buffer solvent systems) or by silica gel chromatography (4:1 CHCl 3 :MeOH). The attachment of sulfonated groups to the β-positions of a tetrapyrrolic macrocycle is an alternative method toward the generation of hydrophilic sulfonated derivatives. This approach was applied to the generation of alkylsulfonated bacteriochlorins [128]. For example, sulfonated bacteriochlorophyll derivatives were prepared by reaction of Pd-bacteriopheophorbide (108) with homotaurine (Scheme 31) [128]. Treatment of either 109 or the sulfo-NHS ester 110 with a second equivalent of homotaurine also yielded the bis-sulfonated product 111 (with the trisulfonated compound arising from imine formation with the β-acetyl group as a minor product). Bacteriochlorin 112M could also prepared using a similar procedure using taurine as the nucleophile. All of the sulfonated derivatives were found to possess high solubility in water (up to 40 mg/mL) [129]. The products were either purified by HPLC (MeOH/phosphate-buffer solvent systems) or by silica gel chromatography (4:1 CHCl3:MeOH).
Sulfonate functionalities may also be introduced at a late stage in the porphyrin synthesis by transition metal-mediated cross-coupling strategies. For instance, Anderson and co-workers introduced sulfonate groups to the meso-positions of a meso-brominated PEGylated conjugated porphyrin dimer using a Suzuki coupling with a sulfonated arylboronic acid, a strategy similar to the introduction of pyridine functionalities described above (cf. Scheme 13) [70]. The tetrasulfonated porphyrin dimer 113 (Figure 7) was purified using semi-preparative reverse-phase HPLC.

Porphyrins with Phosphate/Phosphonate Functional Groups
The introduction of alkylphosphonate functional groups to the periphery of a porphyrin is another strategy to impart hydrophilicity to porphyrins and hydroporphyrins. Phosphate groups have also been employed, but because of the increased hydrolytic lability of the phosphate group, only rarely.
Alkyl phosphonates have been introduced to the porphyrin by modification of a porphyrin or by the synthesis of the porphyrin macrocycle with protected phosphonate/phosphate or alcohol Scheme 31. Sulfonated Pd-bacteriopheophorbide, as described by the group of Scherz [129]. EDC = 1-ethyl-3-(3-dimethylaminopropyl)carbodiimide.
Sulfonate functionalities may also be introduced at a late stage in the porphyrin synthesis by transition metal-mediated cross-coupling strategies. For instance, Anderson and co-workers introduced sulfonate groups to the meso-positions of a meso-brominated PEGylated conjugated porphyrin dimer using a Suzuki coupling with a sulfonated arylboronic acid, a strategy similar to the introduction of pyridine functionalities described above (cf. Scheme 13) [70]. The tetrasulfonated porphyrin dimer 113 (Figure 7) was purified using semi-preparative reverse-phase HPLC. chlorophyll derivatives were prepared by reaction of Pd-bacteriopheophorbide (108) with homotaurine (Scheme 31) [128]. Treatment of either 109 or the sulfo-NHS ester 110 with a second equivalent of homotaurine also yielded the bis-sulfonated product 111 (with the trisulfonated compound arising from imine formation with the β-acetyl group as a minor product). Bacteriochlorin 112M could also prepared using a similar procedure using taurine as the nucleophile. All of the sulfonated derivatives were found to possess high solubility in water (up to 40 mg/mL) [129]. The products were either purified by HPLC (MeOH/phosphate-buffer solvent systems) or by silica gel chromatography (4:1 CHCl3:MeOH).
Sulfonate functionalities may also be introduced at a late stage in the porphyrin synthesis by transition metal-mediated cross-coupling strategies. For instance, Anderson and co-workers introduced sulfonate groups to the meso-positions of a meso-brominated PEGylated conjugated porphyrin dimer using a Suzuki coupling with a sulfonated arylboronic acid, a strategy similar to the introduction of pyridine functionalities described above (cf. Scheme 13) [70]. The tetrasulfonated porphyrin dimer 113 (Figure 7) was purified using semi-preparative reverse-phase HPLC.

Porphyrins with Phosphate/Phosphonate Functional Groups
The introduction of alkylphosphonate functional groups to the periphery of a porphyrin is another strategy to impart hydrophilicity to porphyrins and hydroporphyrins. Phosphate groups have also been employed, but because of the increased hydrolytic lability of the phosphate group, only rarely.
Alkyl phosphonates have been introduced to the porphyrin by modification of a porphyrin or by the synthesis of the porphyrin macrocycle with protected phosphonate/phosphate or alcohol building blocks. Deprotection and subsequent modification of the porphyrin furnished the water-soluble phosphonated derivatives. One of the first examples of porphyrins bearing phosphonate groups was introduced by the group of Montforts [130]. They prepared water-soluble metalloporphyrins by phosphonation of the primary alkyl alcohols in deuteroporphyrin derivative 114M (Scheme 32) [130]. Their strategy involved the conversion of the alcohols in 114M to brominated derivative 115M, followed by reaction with P(OSiMe 3 ) 3 , and subsequent hydrolysis of the intermediate with MeOH/H 2 O to afford phosphonate 116M. The free phosphonate functional groups were used to attach these derivatives to electrode surfaces [130]. Using a similar strategy, diphosphonated chlorin derivatives rac-117 and rac-118 were also prepared (Scheme 32). Along analogous pathways, trans-AB porphyrins bearing amino (121c), acetamido (121d), and iodoacetamido (121e) bioconjugatable tethers at the meso-phenyl position opposite the solubilizing group also became accessible (Scheme 33) [132]. This approach is suitable for the synthesis of phosphonated chlorins, synthesized by using dipyrromethane building block 123, bearing two protected alcohols (Scheme 34) [133]. After condensation of 122 and 123, the benzyl ether protecting groups in 124 were removed, and the alcohols were brominated and phosphonated. The phosphonate ester was then treated with TMS-Br to furnish the free phosphonates. Scheme 32. Phosphonated β-alkyl porphyrin derivatives, as described the group of Montforts [130].
While the requisite alkyl alcohols for phosphonation in 114M were generated by functional group manipulation of the propionic acid side chains present in the natural product precursors, the requisite alcohols can also be introduced (in free or protected form) at the porphyrin synthesis stage. For instance, Lindsey and co-workers prepared trans-AB porphyrin 119 by using a dipyrromethane precursor bearing two t-butyldimethylsilyl-(TBDMS) protected hydroxyl groups (Scheme 33) [131]. After removal of the protecting groups, the hydroxyl groups could be derivatized in a similar manner as described by Montforts [130] to provide the protected phosphonate ester 120. An ester hydrolysis revealed the free phosphonate groups, conveying water-solubility. The corresponding zinc complexes were also prepared.
Along analogous pathways, trans-AB porphyrins bearing amino (121c), acetamido (121d), and iodoacetamido (121e) bioconjugatable tethers at the meso-phenyl position opposite the solubilizing group also became accessible (Scheme 33) [132]. This approach is suitable for the synthesis of phosphonated chlorins, synthesized by using dipyrromethane building block 123, bearing two protected alcohols (Scheme 34) [133]. After condensation of 122 and 123, the benzyl ether protecting groups in 124 were removed, and the alcohols were brominated and phosphonated. The phosphonate ester was then treated with TMS-Br to furnish the free phosphonates. Scheme 32. Phosphonated β-alkyl porphyrin derivatives, as described the group of Montforts [130].
Along analogous pathways, trans-AB porphyrins bearing amino (121c), acetamido (121d), and iodoacetamido (121e) bioconjugatable tethers at the meso-phenyl position opposite the solubilizing group also became accessible (Scheme 33) [132]. This approach is suitable for the synthesis of phosphonated chlorins, synthesized by using dipyrromethane building block 123, bearing two protected alcohols (Scheme 34) [133]. After condensation of 122 and 123, the benzyl ether protecting groups in 124 were removed, and the alcohols were brominated and phosphonated. The phosphonate ester was then treated with TMS-Br to furnish the free phosphonates. Scheme 33. trans-AB Porphyrins bearing swallowtail phosphonate motifs, as described by the group of Lindsey [131,132].
Lindsey and co-workers also prepared trans-AB porphyrins incorporating phosphate groups, though in this instance they started with a dipyrromethane precursor already bearing phosphate esters (Scheme 35) [131]. Hydrolysis of the protected phosphate groups afforded the free phosphate groups. Scheme 33. trans-AB Porphyrins bearing swallowtail phosphonate motifs, as described by the group of Lindsey [131,132]. Scheme 34. Synthetic chlorins bearing phosphonate swallowtail motifs, as described by the group of Lindsey [133]. TMPi = 2,2,6,6-tetramethylpiperidine.
Lindsey and co-workers also prepared trans-AB porphyrins incorporating phosphate groups, though in this instance they started with a dipyrromethane precursor already bearing phosphate esters (Scheme 35) [131]. Hydrolysis of the protected phosphate groups afforded the free phosphate groups. Scheme 34. Synthetic chlorins bearing phosphonate swallowtail motifs, as described by the group of Lindsey [133]. TMPi = 2,2,6,6-tetramethylpiperidine.

Scheme 35.
Porphyrin bearing phosphate swallowtail motif, as described by the group of Lindsey [131].
Phosphonate groups can also be introduced to the porphyrin by starting with dipyrromethane precursors bearing protected phosphonate functional groups. Using this strategy, trans-AB porphyrin 130 ( Figure 8) was synthesized by condensation using a dipyrromethane precursor carrying an 2,6-diphosphonated aryl ring that projects the solubilizing groups above and below the plane of the macrocycle target (cf. Scheme 35) [134]. Hydrolysis of the phosphonate esters and saponification affords the trans-AB porphyrin bearing both the phosphonate solubilization groups and a carboxylic acid bioconjugatable tether. Using a similar strategy as for chlorin 125, this 2,6-aryl-phosphonate motif was also incorporated into chlorin 131 [133]. Again, the Suzuki coupling strategy of βdibromobacteriochlorins proved versatile enough to be applicable to the introduction of β-arylphosphonate groups (cf. Scheme 6) to afford, after hydrolysis of the phosphonate esters, watersoluble bacteriochlorin 132. Phosphonate groups can also be introduced to the porphyrin by starting with dipyrromethane precursors bearing protected phosphonate functional groups. Using this strategy, trans-AB porphyrin 130 ( Figure 8) was synthesized by condensation using a dipyrromethane precursor carrying an 2,6-diphosphonated aryl ring that projects the solubilizing groups above and below the plane of the macrocycle target (cf. Scheme 35) [134]. Hydrolysis of the phosphonate esters and saponification affords the trans-AB porphyrin bearing both the phosphonate solubilization groups and a carboxylic acid bioconjugatable tether. Using a similar strategy as for chlorin 125, this 2,6-aryl-phosphonate motif was also incorporated into chlorin 131 [133]. Again, the Suzuki coupling strategy of β-dibromobacteriochlorins proved versatile enough to be applicable to the introduction of β-aryl-phosphonate groups (cf. Scheme 6) to afford, after hydrolysis of the phosphonate esters, water-soluble bacteriochlorin 132. Scheme 34. Synthetic chlorins bearing phosphonate swallowtail motifs, as described by the group of Lindsey [133]. TMPi = 2,2,6,6-tetramethylpiperidine.

Scheme 35.
Porphyrin bearing phosphate swallowtail motif, as described by the group of Lindsey [131].
Phosphonate groups can also be introduced to the porphyrin by starting with dipyrromethane precursors bearing protected phosphonate functional groups. Using this strategy, trans-AB porphyrin 130 ( Figure 8) was synthesized by condensation using a dipyrromethane precursor carrying an 2,6-diphosphonated aryl ring that projects the solubilizing groups above and below the plane of the macrocycle target (cf. Scheme 35) [134]. Hydrolysis of the phosphonate esters and saponification affords the trans-AB porphyrin bearing both the phosphonate solubilization groups and a carboxylic acid bioconjugatable tether. Using a similar strategy as for chlorin 125, this 2,6-aryl-phosphonate motif was also incorporated into chlorin 131 [133]. Again, the Suzuki coupling strategy of βdibromobacteriochlorins proved versatile enough to be applicable to the introduction of β-arylphosphonate groups (cf. Scheme 6) to afford, after hydrolysis of the phosphonate esters, watersoluble bacteriochlorin 132.

PEGylated Porphyrins
PEGylation has emerged as a strategy for the preparation of neutral water-soluble porphyrins and hydroporphyrins. It has many benefits over traditional means using ionic groups. For instance, PEGylation strategies are more flexible with respect to where in the synthetic sequence they are introduced. This is because the PEG functional group is not very reactive once installed. Unwanted reactivity to form oligomeric species is also suppressed by using heterobifunctional PEG chains, in which one end of the PEG chain often has a methyl cap. PEGylated porphyrins are also much more amenable to traditional aqueous work-up conditions, as they may partition favorably in organic solvents such as CH 2 Cl 2 and EtOAc [135,136]. Often times PEGylated porphyrins can be purified by normal silica-gel chromatography using polar solvents [14,[137][138][139].

Porphyrinoid Macrocycle Total Synthesis Using PEGylated Building Blocks
Despite these advantages, the multistep manipulation of porphyrins with PEG-groups present throughout the synthesis is relatively rare. For instance, Brunner and co-workers presented such an example. They synthesized the A 3 B porphyrin 133 by mixed condensation of two arylaldehydes and pyrrole, with one of the aryl aldehydes carrying a PEG chain (n = 2, 3 or 17) (Scheme 36) [140]. The resulting A 3 B PEGylated porphyrins 133a-133c were purified using ordinary silica gel chromatography (CH 2 Cl 2 /MeOH mixtures). The PEGylated porphyrins were also amenable to further modification at the malonic ester functional group to generate platinum-porphyrin conjugates. and hydroporphyrins. It has many benefits over traditional means using ionic groups. For instance, PEGylation strategies are more flexible with respect to where in the synthetic sequence they are introduced. This is because the PEG functional group is not very reactive once installed. Unwanted reactivity to form oligomeric species is also suppressed by using heterobifunctional PEG chains, in which one end of the PEG chain often has a methyl cap. PEGylated porphyrins are also much more amenable to traditional aqueous work-up conditions, as they may partition favorably in organic solvents such as CH2Cl2 and EtOAc [135,136]. Often times PEGylated porphyrins can be purified by normal silica-gel chromatography using polar solvents [14,[137][138][139].

Porphyrinoid Macrocycle Total Synthesis Using PEGylated Building Blocks
Despite these advantages, the multistep manipulation of porphyrins with PEG-groups present throughout the synthesis is relatively rare. For instance, Brunner and co-workers presented such an example. They synthesized the A3B porphyrin 133 by mixed condensation of two arylaldehydes and pyrrole, with one of the aryl aldehydes carrying a PEG chain (n = 2, 3 or 17) (Scheme 36) [140]. The resulting A3B PEGylated porphyrins 133a-133c were purified using ordinary silica gel chromatography (CH2Cl2/MeOH mixtures). The PEGylated porphyrins were also amenable to further modification at the malonic ester functional group to generate platinum-porphyrin conjugates. Scheme 36. A3B porphyrin carrying three short PEG chains, as described by the group of Brunner [140].
Another example for the early introduction of PEGylated building blocks was reported by the group of Anderson [70]. Using a PEGylated benzaldehyde, porphyrin 26 bearing two methyl-capped tetraethylene glycol (TEG) groups on opposite meso-phenylgroups was prepared. Leaving the PEG chains intact, it was converted to the bis-acetylene linked porphyrin dimer 134. Porphyrin dimer 134 was found not to be sufficiently soluble in aqueous media for biological application. Therefore, these materials were further derivatized with additional solubilizing groups, all while the PEG functional groups remained intact (Scheme 37) [70].
Starting from the meso-dibromo dimer 49, cationic (pyridinium; cf. Scheme 13), anionic (sulfonate) and carboxlyate (cf. Scheme 25) groups were introduced using either Suzuki or Sonogashira coupling strategies. The Senge arylation method was also used to introduce ammonium and pyridyl solubilizing groups (cf. Scheme 7). The dimers were separated by either recrystallization (DMF, Et2O) or by semi-preparative reverse phase HPLC. Due to insufficient solubility of the compounds in regular reverse-phase HPLC solvents (such as CH3CN, MeOH, water), DMF, DMSO, or THF were used. Also due to solubility issues, the authors could not measure logP values for these compounds in octanol:water. However, they did compare the relative polarity of some derivatives by means of their retention times under reverse-phase HPLC conditions (Table 1) Another example for the early introduction of PEGylated building blocks was reported by the group of Anderson [70]. Using a PEGylated benzaldehyde, porphyrin 26 bearing two methyl-capped tetraethylene glycol (TEG) groups on opposite meso-phenylgroups was prepared. Leaving the PEG chains intact, it was converted to the bis-acetylene linked porphyrin dimer 134. Porphyrin dimer 134 was found not to be sufficiently soluble in aqueous media for biological application. Therefore, these materials were further derivatized with additional solubilizing groups, all while the PEG functional groups remained intact (Scheme 37) [70]. PEG-substituted dipyrromethanes also found use in the early introduction of solubilizing groups. The group of Lindsey was able to synthesize chlorins from a PEGylated dipyrromethane precursor (Scheme 38) [136]. This strategy also incorporated a bioconjugatable tether at another meso-position, the precursor of which was also introduced at the dipyrromethane stage.
Scheme 37. Hydrophilic bis-acetylene linked porphyrin dimers carrying PEG chains and various other solubilizing motifs, as described by the group of Anderson [70].
Starting from the meso-dibromo dimer 49, cationic (pyridinium; cf. Scheme 13), anionic (sulfonate) and carboxlyate (cf. Scheme 25) groups were introduced using either Suzuki or Sonogashira coupling strategies. The Senge arylation method was also used to introduce ammonium and pyridyl solubilizing groups (cf. Scheme 7). The dimers were separated by either recrystallization (DMF, Et 2 O) or by semi-preparative reverse phase HPLC. Due to insufficient solubility of the compounds in regular reverse-phase HPLC solvents (such as CH 3 CN, MeOH, water), DMF, DMSO, or THF were used. Also due to solubility issues, the authors could not measure logP values for these compounds in octanol:water. However, they did compare the relative polarity of some derivatives by means of their retention times under reverse-phase HPLC conditions (Table 1). PEG-substituted dipyrromethanes also found use in the early introduction of solubilizing groups. The group of Lindsey was able to synthesize chlorins from a PEGylated dipyrromethane precursor (Scheme 38) [136]. This strategy also incorporated a bioconjugatable tether at another meso-position, the precursor of which was also introduced at the dipyrromethane stage. PEG-substituted dipyrromethanes also found use in the early introduction of solubilizing groups. The group of Lindsey was able to synthesize chlorins from a PEGylated dipyrromethane precursor (Scheme 38) [136]. This strategy also incorporated a bioconjugatable tether at another meso-position, the precursor of which was also introduced at the dipyrromethane stage. Scheme 38. PEGylated synthetic chlorins using PEGylated building blocks, as described by the group of Lindsey [136]. TMPi = 2,2,6,6-tetramethylpiperidine. Scheme 38. PEGylated synthetic chlorins using PEGylated building blocks, as described by the group of Lindsey [136]. TMPi = 2,2,6,6-tetramethylpiperidine.

PEGylation of meso-aryl Porphyrins
A number of meso-tetraarylporphyrins bearing PEG groups have been synthesized by PEGylation of porphyrins incorporating suitable linker functionalities on the aryl groups. These porphyrins are usually prepared via Adler or Lindsey methods and the PEG groups can be linked by various methods including etherification, amidation or esterification reactions. Particularly popular linking groups for the PEGylation of porphyrins are meso-phenol substituents. PEGylation of various meso-tetrahydroxyphenyl porphyrin derivatives with a suitably functionalized PEG precursor yields water-soluble porphyrins, with activation of the PEG group often required.

PEGylation of meso-aryl Porphyrins
A number of meso-tetraarylporphyrins bearing PEG groups have been synthesized by PEGylation of porphyrins incorporating suitable linker functionalities on the aryl groups. These porphyrins are usually prepared via Adler or Lindsey methods and the PEG groups can be linked by various methods including etherification, amidation or esterification reactions. Particularly popular linking groups for the PEGylation of porphyrins are meso-phenol substituents. PEGylation of various mesotetrahydroxyphenyl porphyrin derivatives with a suitably functionalized PEG precursor yields water-soluble porphyrins, with activation of the PEG group often required.

meso-Tetrakis(4-hydroxyphenyl)porphyrin
Under similar conditions, single PEG chains or PEG-dendrimers (Scheme 41) [142] can also be introduced into asymmetric meso-hydroxyphenylporphyrins [143,144]. Vitalini and co-workers prepared PEGylated derivatives of 76 by alkylation of the phenolic oxygens with a chlorinated PEG [145]. The PEG-functionalized porphyrins could be purified by adding a solution of the compound in CH2Cl2 to a cold solution of Et2O to induce precipitation (for larger PEGs) [137,143]; porphyrins bearing smaller PEG-chains could also be purified by column chromatography (CH2Cl2-acetone-MeOH or CH2Cl2/EtOH mixtures) [137,142]. Scheme 39. PEGylated derivatives of meso-tetrakis(3-hydroxyphenyl)chlorin, as described by the group of Sinn [141]. meso-Tetrakis(4-hydroxyphenyl)porphyrin (76) can also be alkylated using various activated PEGs. For instance, this procedure has been employed to alkylate 76 by treatment with PEG-mesylates to form 144. (Scheme 40) [137]. PEGylation of meso-arylporphyrins was also achieved by inversion of the Williamson ether synthesis reaction partners, i.e., involving a halogenated porphyrin precursor and PEGs bearing a Under similar conditions, single PEG chains or PEG-dendrimers (Scheme 41) [142] can also be introduced into asymmetric meso-hydroxyphenylporphyrins [143,144]. Vitalini and co-workers prepared PEGylated derivatives of 76 by alkylation of the phenolic oxygens with a chlorinated PEG [145]. The PEG-functionalized porphyrins could be purified by adding a solution of the compound in CH 2 Cl 2 to a cold solution of Et 2 O to induce precipitation (for larger PEGs) [137,143]; porphyrins bearing smaller PEG-chains could also be purified by column chromatography (CH 2 Cl 2 -acetone-MeOH or CH 2 Cl 2 /EtOH mixtures) [137,142]. Scheme 40. PEGylated derivatives of meso-tetra(4-hydroxyphenyl)porphyrin, as described by the group of Pozzi [137].

Scheme 41.
Amphiphilic porphyrin with a PEG-dendrimer, as described by the group of Dumoulin [142].
PEGylation of meso-arylporphyrins was also achieved by inversion of the Williamson ether synthesis reaction partners, i.e., involving a halogenated porphyrin precursor and PEGs bearing a free alcohol. An example is the PEGylation of tetra(p-bromomethylphenyl)porphyrin (147) with a methyl-capped PEG alcohol (Mn = 550) that afforded the tetra-PEGylated porphyrin 148 as the main product, along with partially PEGylated porphyrins (Scheme 42). The porphyrin starting material was prepared by Lindsey porphyrin synthesis from 4-(bromomethyl)benzaldehyde and pyrrole [146]. The PEGylated products were amenable to aqueous work-up (extraction with CH2Cl2) and were purified by HPLC. Scheme 42. PEGylated meso-aryl porphyrins by benzylation of a PEG with tetra(p-bromomethylphenyl) porphyrin, as described by the group of Lee [146]. PEGylation of meso-arylporphyrins was also achieved by inversion of the Williamson ether synthesis reaction partners, i.e., involving a halogenated porphyrin precursor and PEGs bearing a free alcohol. An example is the PEGylation of tetra(p-bromomethylphenyl)porphyrin (147) with a methyl-capped PEG alcohol (M n = 550) that afforded the tetra-PEGylated porphyrin 148 as the main product, along with partially PEGylated porphyrins (Scheme 42). The porphyrin starting material was prepared by Lindsey porphyrin synthesis from 4-(bromomethyl)benzaldehyde and pyrrole [146]. The PEGylated products were amenable to aqueous work-up (extraction with CH 2 Cl 2 ) and were purified by HPLC. Scheme 40. PEGylated derivatives of meso-tetra(4-hydroxyphenyl)porphyrin, as described by the group of Pozzi [137].

Scheme 41.
Amphiphilic porphyrin with a PEG-dendrimer, as described by the group of Dumoulin [142].
PEGylation of meso-arylporphyrins was also achieved by inversion of the Williamson ether synthesis reaction partners, i.e., involving a halogenated porphyrin precursor and PEGs bearing a free alcohol. An example is the PEGylation of tetra(p-bromomethylphenyl)porphyrin (147) with a methyl-capped PEG alcohol (Mn = 550) that afforded the tetra-PEGylated porphyrin 148 as the main product, along with partially PEGylated porphyrins (Scheme 42). The porphyrin starting material was prepared by Lindsey porphyrin synthesis from 4-(bromomethyl)benzaldehyde and pyrrole [146]. The PEGylated products were amenable to aqueous work-up (extraction with CH2Cl2) and were purified by HPLC. Scheme 42. PEGylated meso-aryl porphyrins by benzylation of a PEG with tetra(p-bromomethylphenyl) porphyrin, as described by the group of Lee [146]. PEGylated meso-aryl porphyrins by benzylation of a PEG with tetra(p-bromomethylphenyl)porphyrin, as described by the group of Lee [146]. meso-Aryl porphyrins bearing peripheral carboxylic acid functional groups can be PEGylated by amide formation using an amine-terminated PEG. For instance, Scolaro and co-workers prepared PEGylated derivatives of meso-tetrakis(4-carboxyphenyl)porphyrin (149) by treatment with Jeffamine M-600 (n = 7-9) (Scheme 43) [147].
Also starting from tetraacid 149, Lovell and co-workers reacted it with a variety of homobi-functional PEG-diamines (average Mw ranging from 150 Da to 10 kDa) to synthesize a PEG-linked porphyrin mesh 151 (Figure 9) [148]. This reaction illustrates the complex cross-linked structure formed when using PEGs capable of reacting at both ends. The porphyrin-PEG-mesh was purified by dialysis, followed by addition of citric acid to precipitate unreacted porphyrin.
PEGylated porphyrins and hydroporphyrins with amide linkages can also be prepared starting with aminophenyl porphyrins. For instance, Peng et al. functionalized a chlorin with a poly-(ε-caprolactone)-polyethyleneglycol) diblock copolymer [149]. Introduction of the PEG-polymer was achieved by treatment of meso-tetrakis(4-aminophenyl)chlorin with the acid chloride of the diblock copolymer. The polymer-functionalized porphyrin was purified by precipitation with Et 2 O, followed by a dialysis step in acetone. Vicente and co-workers prepared water-soluble porphyrin-peptide conjugates with a PEG linker on one meso-aryl group starting from an AB 3 porphyrin 152 bearing one p-aminophenyl group. meso-Aryl porphyrins bearing peripheral carboxylic acid functional groups can be PEGylated by amide formation using an amine-terminated PEG. For instance, Scolaro and co-workers prepared PEGylated derivatives of meso-tetrakis(4-carboxyphenyl)porphyrin (149) by treatment with Jeffamine M-600 (n = 7-9) (Scheme 43) [147]. Scheme 43. PEGylated porphyrins derived from meso-tetrakis(4-carboxyphenyl)porphyrin using a PEG-amine, as described by the group of Scolaro [147].
Also starting from tetraacid 149, Lovell and co-workers reacted it with a variety of homobifunctional PEG-diamines (average Mw ranging from 150 Da to 10 kDa) to synthesize a PEG-linked porphyrin mesh 151 (Figure 9) [148]. This reaction illustrates the complex cross-linked structure formed when using PEGs capable of reacting at both ends. The porphyrin-PEG-mesh was purified by dialysis, followed by addition of citric acid to precipitate unreacted porphyrin. PEGylated porphyrins and hydroporphyrins with amide linkages can also be prepared starting with aminophenyl porphyrins. For instance, Peng et al. functionalized a chlorin with a poly-(εcaprolactone)-polyethyleneglycol) diblock copolymer [149]. Introduction of the PEG-polymer was Scheme 43. PEGylated porphyrins derived from meso-tetrakis(4-carboxyphenyl)porphyrin using a PEG-amine, as described by the group of Scolaro [147]. meso-Aryl porphyrins bearing peripheral carboxylic acid functional groups can be PEGylated by amide formation using an amine-terminated PEG. For instance, Scolaro and co-workers prepared PEGylated derivatives of meso-tetrakis(4-carboxyphenyl)porphyrin (149) by treatment with Jeffamine M-600 (n = 7-9) (Scheme 43) [147]. Scheme 43. PEGylated porphyrins derived from meso-tetrakis(4-carboxyphenyl)porphyrin using a PEG-amine, as described by the group of Scolaro [147].
Also starting from tetraacid 149, Lovell and co-workers reacted it with a variety of homobifunctional PEG-diamines (average Mw ranging from 150 Da to 10 kDa) to synthesize a PEG-linked porphyrin mesh 151 (Figure 9) [148]. This reaction illustrates the complex cross-linked structure formed when using PEGs capable of reacting at both ends. The porphyrin-PEG-mesh was purified by dialysis, followed by addition of citric acid to precipitate unreacted porphyrin. PEGylated porphyrins and hydroporphyrins with amide linkages can also be prepared starting with aminophenyl porphyrins. For instance, Peng et al. functionalized a chlorin with a poly-(εcaprolactone)-polyethyleneglycol) diblock copolymer [149]. Introduction of the PEG-polymer was The amine functionality in 152 was reacted with diglycolic anhydride, followed by amide-coupling using a PEG-amine and Boc-deprotection (Scheme 44). A peptidyl resin can be coupled to the hydroxybenzotriazole (HOBt) ester of the porphyrin 154 [150]. More hydrophilic PEGylated A 3 B porphyrins bearing three carboxyphenyl groups were also prepared in a similar manner [150]. Oligo-ethylene glycol amide-linkages have also been utilized as hydrophilic spacers in instances that require designed structures on the periphery of a hydrophilic porphyrin. Using this strategy, Alessio and co-workers have prepared ruthenium-porphyrin conjugates with oligoethylene glycol spacers [151]. This methodology has also been used to develop Rhenium (I)-porphyrin conjugates in a similar manner [152]. require designed structures on the periphery of a hydrophilic porphyrin. Using this strategy, Alessio and co-workers have prepared ruthenium-porphyrin conjugates with oligoethylene glycol spacers [151]. This methodology has also been used to develop Rhenium (I)-porphyrin conjugates in a similar manner [152].
Lastly, PEGylation of meso-hydroxyphenylporphyrins can be achieved utilizing ester linkages. Thus, Diederich and co-workers prepared dendritic porphyrin 156 by esterification of porphyrin tetraol 155 with a carboxylic acid-functionalized dendron under Mitsunobu conditions (Scheme 45) [153]. The extension of the reactive alcohol site from the phenolic position using an alkyl chain was employed to accommodate the bulky PEG-dendrimer substituents. The resulting porphyrin-dendrimers were purified by preparative gel permeation chromatography and were soluble in phosphate buffer Lastly, PEGylation of meso-hydroxyphenylporphyrins can be achieved utilizing ester linkages. Thus, Diederich and co-workers prepared dendritic porphyrin 156 by esterification of porphyrin tetraol 155 with a carboxylic acid-functionalized dendron under Mitsunobu conditions (Scheme 45) [153].
The amine functionality in 152 was reacted with diglycolic anhydride, followed by amidecoupling using a PEG-amine and Boc-deprotection (Scheme 44). A peptidyl resin can be coupled to the hydroxybenzotriazole (HOBt) ester of the porphyrin 154 [150]. More hydrophilic PEGylated A3B porphyrins bearing three carboxyphenyl groups were also prepared in a similar manner [150]. Oligoethylene glycol amide-linkages have also been utilized as hydrophilic spacers in instances that require designed structures on the periphery of a hydrophilic porphyrin. Using this strategy, Alessio and co-workers have prepared ruthenium-porphyrin conjugates with oligoethylene glycol spacers [151]. This methodology has also been used to develop Rhenium (I)-porphyrin conjugates in a similar manner [152].
Lastly, PEGylation of meso-hydroxyphenylporphyrins can be achieved utilizing ester linkages. Thus, Diederich and co-workers prepared dendritic porphyrin 156 by esterification of porphyrin tetraol 155 with a carboxylic acid-functionalized dendron under Mitsunobu conditions (Scheme 45) [153]. The extension of the reactive alcohol site from the phenolic position using an alkyl chain was employed to accommodate the bulky PEG-dendrimer substituents. The resulting porphyrin-dendrimers were purified by preparative gel permeation chromatography and were soluble in phosphate buffer The extension of the reactive alcohol site from the phenolic position using an alkyl chain was employed to accommodate the bulky PEG-dendrimer substituents. The resulting porphyrin-dendrimers were purified by preparative gel permeation chromatography and were soluble in phosphate buffer at pH 7. Alternatively, the PEGylation of a meso-hydroxphenyl A 2 B 2 porphyrin by DCC/DMAP-mediated esterification with a PEG-carboxylic acid (1000 Da) was reported (Scheme 46) [154].
π-Extended porphyrin derivatives may also be subjected to the same PEGylation strategies as seen for regular porphyrins. For instance, PEGylation of the phenolic oxygens in quinoline-annulated porphyrin 160 was reported by Luciano et al. (Scheme 47) [14] using a similar O-alkylation method as described for regular porphyrins (Scheme 40).
Precursor porphyrin 159 was prepared from meso-tetrakis(4-methoxyphenyl)porphyrin. A BBr 3 -mediated deprotection was employed to deprotect the phenolic oxygens as the penultimate step of the synthesis. The phenol could then be PEGylated using either a short (n = 4) or long chain (avg. MW 550, n ≈ 12) PEG-mesylate [14]. The short PEG chain derivative 161a was found to be only slightly soluble in water. However, the derivative bearing long PEGs (161b) was soluble in PBS to form~30 mM solutions and were used as photoacoustic imaging contrast agents for in vivo imaging of tumors in a mouse model [14]. π-Extended porphyrin derivatives may also be subjected to the same PEGylation strategies as seen for regular porphyrins. For instance, PEGylation of the phenolic oxygens in quinoline-annulated Scheme 47. PEGylated quinoline-annulated porphyrins, as described by the group of Brückner [14].
Precursor porphyrin 159 was prepared from meso-tetrakis(4-methoxyphenyl)porphyrin. A BBr3mediated deprotection was employed to deprotect the phenolic oxygens as the penultimate step of the synthesis. The phenol could then be PEGylated using either a short (n = 4) or long chain (avg. MW 550, n ≈ 12) PEG-mesylate [14]. The short PEG chain derivative 161a was found to be only slightly soluble in water. However, the derivative bearing long PEGs (161b) was soluble in PBS to form ~30 mM solutions and were used as photoacoustic imaging contrast agents for in vivo imaging of tumors in a mouse model [14].
Brückner and co-workers were able to take advantage of the well-known SNAr reactivity of mesopentafluorophenylporphyrins toward nucleophiles at the p-F positions to introduce PEG groups to pyrrole-modified porphyrins (PMPs) at a late stage of the synthetic sequence toward meso-arylmetalloporpholactones [138,139,155]  Scheme 46. PEGylated A 2 B 2 porphyrin, as described by the group of Nawaz [154]. DCC = dicyclo-hexylcarbodiimide, DMAP = 4-dimethylaminopyridine.
π-Extended porphyrin derivatives may also be subjected to the same PEGylation strategies as seen for regular porphyrins. For instance, PEGylation of the phenolic oxygens in quinoline-annulated porphyrin 160 was reported by Luciano et al. (Scheme 47) [14] using a similar O-alkylation method as described for regular porphyrins (Scheme 40). Scheme 47. PEGylated quinoline-annulated porphyrins, as described by the group of Brückner [14].
Precursor porphyrin 159 was prepared from meso-tetrakis(4-methoxyphenyl)porphyrin. A BBr3mediated deprotection was employed to deprotect the phenolic oxygens as the penultimate step of the synthesis. The phenol could then be PEGylated using either a short (n = 4) or long chain (avg. MW 550, n ≈ 12) PEG-mesylate [14]. The short PEG chain derivative 161a was found to be only slightly soluble in water. However, the derivative bearing long PEGs (161b) was soluble in PBS to form ~30 mM solutions and were used as photoacoustic imaging contrast agents for in vivo imaging of tumors in a mouse model [14].
Brückner and co-workers were able to take advantage of the well-known SNAr reactivity of mesopentafluorophenylporphyrins toward nucleophiles at the p-F positions to introduce PEG groups to pyrrole-modified porphyrins (PMPs) at a late stage of the synthetic sequence toward meso-arylmetalloporpholactones [138,139,155]  Brückner and co-workers were able to take advantage of the well-known S N Ar reactivity of meso-pentafluorophenylporphyrins toward nucleophiles at the p-F positions to introduce PEG groups to pyrrole-modified porphyrins (PMPs) at a late stage of the synthetic sequence toward meso-arylmetalloporpholactones [138,139,155] (Scheme 48). This allowed the preparation of a variety of PEGylated porpholactone metal complexes (163M) that were used as optical high pH or cyanide sensors in water [139]. The PEGylated derivatives were purified by silica gel chromatography (CH 2 Cl 2 /5% MeOH). Similarly, thiol-functionalized sugars were introduced into meso-pentafluorophenylporphyrins using the S N Ar reaction, also resulting in their solubilization in aqueous solutions [156].
Building on previous efforts for the solubilization of antimony porphyrins by axial ligand exchange with alcohols (cf. Scheme 11), Yasuda and co-workers prepared hydrophilic PEGylated phosphorus porphyrins, such as tetraphenylporphyrin derivative 164 ( Figure 10) by introduction of short PEGs as axial ligands. Incorporation of the axial-PEGs furnished highly water-soluble derivatives. Porphyrin 164, for example, has a water-solubility of 17.3 mM [90]. in water [139]. The PEGylated derivatives were purified by silica gel chromatography (CH2Cl2/5% MeOH). Similarly, thiol-functionalized sugars were introduced into meso-pentafluorophenylporphyrins using the SNAr reaction, also resulting in their solubilization in aqueous solutions [156].
Building on previous efforts for the solubilization of antimony porphyrins by axial ligand exchange with alcohols (cf. Scheme 11), Yasuda and co-workers prepared hydrophilic PEGylated phosphorus porphyrins, such as tetraphenylporphyrin derivative 164 ( Figure 10) by introduction of short PEGs as axial ligands. Incorporation of the axial-PEGs furnished highly water-soluble derivatives. Porphyrin 164, for example, has a water-solubility of 17.3 mM [90].

Porphyrins PEGylated at Their β-Positions
A number of PEGylated β-alkyl-porphyrins and -chlorins were prepared. Representative of these are a number of PEGylated chlorin e6 derivatives, prepared firstly by Hamblin et al. [157]. The PEGylation increased tumor targeting of the photosensitizer. Mono-(165a), di-(165b), and tri-(165c) PEGylated derivatives of chlorin e6 were also prepared in which the PEG groups were introduced by esterification at one to three of its carboxylic acids using a short methyl-capped PEG (Scheme 49) [158]. Longer reaction times were needed to increase the yield of the tri-PEGylated product 165c. The authors also measured the solubility of the compounds to be 1.8 ± 1.3 mM for 11, 2.3 ± 1.0 mM for 165a, 3.3 ± 0.9 mM for 165b, and 3.9 ± 0.8 mM for 165c in 1% (v/v) DMSO/water, indicating the increased aqueous solubility with the increase of the number of PEG chains. Products 165a and 165b are single isomers, indicating a sterics-controlled regioselectivity of the sequential PEGylation.
The propionic side chains in protoporphyrin 166 could also be functionalized with PEG-chains through amide linkages, whereby a short diamine established the requisite amine linkage sites. Amine intermediate 167 was then reacted with succinimidyl-PEG5000 to afford the water-soluble PEGylated protoporphyrin derivative 168 (Scheme 50), and its zinc complex [159,160].
Other PEGylated porphyrins were prepared using ether linkages. For example, brominated hematoporphyrin derivative 169 was converted to the corresponding PEGylated compounds 170a-170f by treatment with a stoichiometric excess of a methyl-capped PEG (Scheme 51) [161,162]. Concomitantly, the propionic acid side chains were also derivatized with PEG chains. After hydrolysis of the propionic ester side chains, platinum-conjugates were prepared and evaluated for their antitumor phototoxicty and cytotoxicity [161,162]. The PEGylated derivatives were amenable to aqueous workup and purified by alumina chromatography. Scheme 48. PEGylated porpholactone derived from meso-tetrakis(pentafluorophenyl)porphyrin derivatives, as described by the group of Brückner [139].
Building on previous efforts for the solubilization of antimony porphyrins by axial ligand exchange with alcohols (cf. Scheme 11), Yasuda and co-workers prepared hydrophilic PEGylated phosphorus porphyrins, such as tetraphenylporphyrin derivative 164 ( Figure 10) by introduction of short PEGs as axial ligands. Incorporation of the axial-PEGs furnished highly water-soluble derivatives. Porphyrin 164, for example, has a water-solubility of 17.3 mM [90].

Porphyrins PEGylated at Their β-Positions
A number of PEGylated β-alkyl-porphyrins and -chlorins were prepared. Representative of these are a number of PEGylated chlorin e6 derivatives, prepared firstly by Hamblin et al. [157]. The PEGylation increased tumor targeting of the photosensitizer. Mono-(165a), di-(165b), and tri-(165c) PEGylated derivatives of chlorin e6 were also prepared in which the PEG groups were introduced by esterification at one to three of its carboxylic acids using a short methyl-capped PEG (Scheme 49) [158]. Longer reaction times were needed to increase the yield of the tri-PEGylated product 165c. The authors also measured the solubility of the compounds to be 1.8 ± 1.3 mM for 11, 2.3 ± 1.0 mM for 165a, 3.3 ± 0.9 mM for 165b, and 3.9 ± 0.8 mM for 165c in 1% (v/v) DMSO/water, indicating the increased aqueous solubility with the increase of the number of PEG chains. Products 165a and 165b are single isomers, indicating a sterics-controlled regioselectivity of the sequential PEGylation.
The propionic side chains in protoporphyrin 166 could also be functionalized with PEG-chains through amide linkages, whereby a short diamine established the requisite amine linkage sites. Amine intermediate 167 was then reacted with succinimidyl-PEG5000 to afford the water-soluble PEGylated protoporphyrin derivative 168 (Scheme 50), and its zinc complex [159,160].
Other PEGylated porphyrins were prepared using ether linkages. For example, brominated hematoporphyrin derivative 169 was converted to the corresponding PEGylated compounds 170a-170f by treatment with a stoichiometric excess of a methyl-capped PEG (Scheme 51) [161,162]. Concomitantly, the propionic acid side chains were also derivatized with PEG chains. After hydrolysis of the propionic ester side chains, platinum-conjugates were prepared and evaluated for their antitumor phototoxicty and cytotoxicity [161,162]. The PEGylated derivatives were amenable to aqueous workup and purified by alumina chromatography.

Porphyrins PEGylated at Their β-Positions
A number of PEGylated β-alkyl-porphyrins and -chlorins were prepared. Representative of these are a number of PEGylated chlorin e6 derivatives, prepared firstly by Hamblin et al. [157]. The PEGylation increased tumor targeting of the photosensitizer. Mono-(165a), di-(165b), and tri-(165c) PEGylated derivatives of chlorin e6 were also prepared in which the PEG groups were introduced by esterification at one to three of its carboxylic acids using a short methyl-capped PEG (Scheme 49) [158]. Longer reaction times were needed to increase the yield of the tri-PEGylated product 165c. The authors also measured the solubility of the compounds to be 1.8 ± 1.3 mM for 11, 2.3 ± 1.0 mM for 165a, 3.3 ± 0.9 mM for 165b, and 3.9 ± 0.8 mM for 165c in 1% (v/v) DMSO/water, indicating the increased aqueous solubility with the increase of the number of PEG chains. Products 165a and 165b are single isomers, indicating a sterics-controlled regioselectivity of the sequential PEGylation. The propionic side chains in protoporphyrin 166 could also be functionalized with PEG-chains through amide linkages, whereby a short diamine established the requisite amine linkage sites. Amine intermediate 167 was then reacted with succinimidyl-PEG 5000 to afford the water-soluble PEGylated protoporphyrin derivative 168 (Scheme 50), and its zinc complex [159,160]. Scheme 49. PEGylated derivatives of chlorin e6, as described by the group of Greer [158]. EDC = 1-ethyl3-(3-dimethylaminopropyl)carbodiimide, DMAP = 4-dimethylaminopyridine.
Scheme 50. PEGylated protoporphyrin and its zinc complex, as described by the group of Maeda [159].
Etherification conditions were also applied to cycloimide-bacteriochlorin alcohol derivative 171 (Scheme 52) [163]. Activation of the hydroxyethyl substituent on the bacteriochlorin 171 with trifluoroacetic anhydride, followed by treatment with hydroxyl-terminated short PEGs and diols of varying length gave the corresponding derivatives 172a-172d. The products were insoluble in water, but aqueous solutions were prepared with the help of 10% Cremophore EL ® , a PEGylated castor oil formulation vehicle. Other PEGylated porphyrins were prepared using ether linkages. For example, brominated hematoporphyrin derivative 169 was converted to the corresponding PEGylated compounds 170a-170f by treatment with a stoichiometric excess of a methyl-capped PEG (Scheme 51) [161,162]. Concomitantly, the propionic acid side chains were also derivatized with PEG chains. After hydrolysis of the propionic ester side chains, platinum-conjugates were prepared and evaluated for their antitumor phototoxicty and cytotoxicity [161,162]. The PEGylated derivatives were amenable to aqueous work-up and purified by alumina chromatography. Scheme 49. PEGylated derivatives of chlorin e6, as described by the group of Greer [158]. EDC = 1-ethyl3-(3-dimethylaminopropyl)carbodiimide, DMAP = 4-dimethylaminopyridine.
Etherification conditions were also applied to cycloimide-bacteriochlorin alcohol derivative 171 (Scheme 52) [163]. Activation of the hydroxyethyl substituent on the bacteriochlorin 171 with trifluoroacetic anhydride, followed by treatment with hydroxyl-terminated short PEGs and diols of varying length gave the corresponding derivatives 172a-172d. The products were insoluble in water, but aqueous solutions were prepared with the help of 10% Cremophore EL ® , a PEGylated castor oil formulation vehicle. Etherification conditions were also applied to cycloimide-bacteriochlorin alcohol derivative 171 (Scheme 52) [163]. Activation of the hydroxyethyl substituent on the bacteriochlorin 171 with trifluoroacetic anhydride, followed by treatment with hydroxyl-terminated short PEGs and diols of varying length gave the corresponding derivatives 172a-172d. The products were insoluble in water, but aqueous solutions were prepared with the help of 10% Cremophore EL ® , a PEGylated castor oil formulation vehicle. The meso-Suzuki coupling method developed by Lindsey and co-workers and utilized for the introduction of a variety of solubilization groups to hydroporphyrins (cf. Schemes 5, 12 and 26) was also utilized for the introduction of PEG groups to bacteriochlorin 173 (Scheme 53) [164]. Bacteriochlorin 173 was prepared by Suzuki coupling of the corresponding meso-bromobacteriochlorin with an aryl-boronic ester bearing two unprotected aldehyde functional groups. The aldehyde functionalities were PEGylated by reductive amination with an amine-terminated PEG to afford the water-soluble PEGylated bacteriochlorin 174.  The meso-Suzuki coupling method developed by Lindsey and co-workers and utilized for the introduction of a variety of solubilization groups to hydroporphyrins (cf. Schemes 5,12 and 26) was also utilized for the introduction of PEG groups to bacteriochlorin 173 (Scheme 53) [164].
Bacterio-chlorin 173 was prepared by Suzuki coupling of the corresponding meso-bromobacteriochlorin with an aryl-boronic ester bearing two unprotected aldehyde functional groups. The aldehyde functionalities were PEGylated by reductive amination with an amine-terminated PEG to afford the water-soluble PEGylated bacteriochlorin 174. Scheme 52. Hydrophilic bacteriochlorin cycloimides, as described by the group of Feofanov [163].
The meso-Suzuki coupling method developed by Lindsey and co-workers and utilized for the introduction of a variety of solubilization groups to hydroporphyrins (cf. Schemes 5, 12 and 26) was also utilized for the introduction of PEG groups to bacteriochlorin 173 (Scheme 53) [164]. Bacteriochlorin 173 was prepared by Suzuki coupling of the corresponding meso-bromobacteriochlorin with an aryl-boronic ester bearing two unprotected aldehyde functional groups. The aldehyde functionalities were PEGylated by reductive amination with an amine-terminated PEG to afford the water-soluble PEGylated bacteriochlorin 174. Scheme 53. PEGylated bacteriochlorins formed by reductive amination, as described by the group of Lindsey [164].
Another representative example for the introduction of PEG groups via Suzuki coupling of dibromobacteriochlorin 19 with a Boc-protected amine-derivatized boronic ester, followed by Bocdeprotection under standard conditions, afforded diaryl bacteriochlorin 175 carrying two amine groups. The amines were PEGylated by amide formation with a PEG-NHS ester to afford bacteriochlorin 176 (Scheme 54) [135]. Derivatives bearing bioconjugatable tethers (177) and (178) were also prepared using a regioselective meso-bromination strategy, followed by similar coupling sequences [135].
The products were compared by Lindsey and co-workers according to several notable parameters [65] ( Table 2). The method of purification of the water-soluble adducts, the solubility of the compounds (as measured by the change in UV-vis absorption spectra over a 1000-fold concentration range), the full width at half-maximum (FWHM) of the longest wavelength of absorption and emission, and the stability of the chromophores in the light and dark.Overall, it was found that either the cationic ammonium or neutral-PEGylated species were the most promising derivatives because of their facile purification (precipitation), their amenability to further bioconjugation reactions, and good dark and light stabilities. The PEGylated derivatives were also shown to display very little aggregation, as demonstrated by the sharp absorbance and emission peaks in their optical spectra over a 1000-fold concentration range. Another representative example for the introduction of PEG groups via Suzuki coupling of dibromobacteriochlorin 19 with a Boc-protected amine-derivatized boronic ester, followed by Boc-deprotection under standard conditions, afforded diaryl bacteriochlorin 175 carrying two amine groups. The amines were PEGylated by amide formation with a PEG-NHS ester to afford bacteriochlorin 176 (Scheme 54) [135]. Derivatives bearing bioconjugatable tethers (177) and (178) were also prepared using a regioselective meso-bromination strategy, followed by similar coupling sequences [135]. Scheme 54. β-Substituted PEGylated synthetic bacteriochlorins via Suzuki coupling, as described by the group of Lindsey [135]. Due to the versatility of the 3,13-dibromobacteriochlorin building block 19, various solubilization motifs could be introduced to this scaffold. Thus, ammonium (compounds 22 and 23, Figure 11), carboxylate (compound 92, Figure 11), phosphonate (compound 132, Figure 11) and PEG (compound 176, Figure 11) solubilizing motifs were introduced by coupling with suitable arylboronic esters as shown in Scheme 54. Scheme 54. β-Substituted PEGylated synthetic bacteriochlorins via Suzuki coupling, as described by the group of Lindsey [135].  The products were compared by Lindsey and co-workers according to several notable parameters [65] ( Table 2). The method of purification of the water-soluble adducts, the solubility of the compounds (as measured by the change in UV-vis absorption spectra over a 1000-fold concentration range), the full width at half-maximum (FWHM) of the longest wavelength of absorption and emission, and the stability of the chromophores in the light and dark.Overall, it was found that either the cationic ammonium or neutral-PEGylated species were the most promising derivatives because of their facile purification (precipitation), their amenability to further bioconjugation reactions, and good dark and light stabilities. The PEGylated derivatives were also shown to display very little aggregation, as demonstrated by the sharp absorbance and emission peaks in their optical spectra over a 1000-fold concentration range.
With the PEGylated derivatives appearing to be among the most promising motifs for solubilization, Lindsey and co-workers set out to prepare a series of PEGylated chlorins and bacteriochlorins (with options for bioconjugation) using a range of synthetic methodologies [135,136]. One such example for the direct, late-stage PEGylation of chlorin derivatives was the azide-alkyne Huisgen-cycloaddition (click) reaction between an alkyne-substituted porphyrin or chlorin and an azide-terminated PEG.
This strategy was employed to perform a direct PEGylation of trans-AB porphyrin 179 (Scheme 55) to afford the PEGylated porphyrin 180 [165]. Along analogous routes, synthetic chlorins 181 and 182 were prepared from alkyne-substituted meso-aryl groups and subsequent reactions with PEG-azides [136]. In addition, an aldol condensation method was developed to directly introduce an aryl group bearing three PEG chains to the β-positions of a β-diacetyl-substituted chlorin 183. Reaction of 183 with a PEG-substituted aryl aldehyde formed the porphyrin-chalcone 184 (Scheme 56) [136]. The absorption spectrum of the PEGylated chlorin-chalcone 184 was broadened in pure water, indicating its aggregation. a For the final step of the synthesis; b measured in aqueous media (PBs except 176, water) by the absorption upon reciprocal change in concentration and path length; c 1 μM in PBS. FWHM = full width at half maximum of the longest wavelength band of absorption or emission, an indicator of aggregation; d The % remaining of a 1 μM solution in PBS after several hours of absorption and fluorescence studies. e The % remaining of a, 1 μM solution in PBS allowed to stand in the dark at 4 °C for 48 h (as determined by absorption intensity of Qy band. With the PEGylated derivatives appearing to be among the most promising motifs for solubilization, Lindsey and co-workers set out to prepare a series of PEGylated chlorins and bacteriochlorins (with options for bioconjugation) using a range of synthetic methodologies [135,136]. One such example for the direct, late-stage PEGylation of chlorin derivatives was the azide-alkyne Huisgen-cycloaddition (click) reaction between an alkyne-substituted porphyrin or chlorin and an azide-terminated PEG.
This strategy was employed to perform a direct PEGylation of trans-AB porphyrin 179 (Scheme 55) to afford the PEGylated porphyrin 180 [165]. Along analogous routes, synthetic chlorins 181 and 182 were prepared from alkyne-substituted meso-aryl groups and subsequent reactions with PEG-azides [136]. In addition, an aldol condensation method was developed to directly introduce an aryl group bearing three PEG chains to the β-positions of a β-diacetyl-substituted chlorin 183. Reaction of 183 with a PEG-substituted aryl aldehyde formed the porphyrin-chalcone 184 (Scheme 56) [136]. The absorption spectrum of the PEGylated chlorin-chalcone 184 was broadened in pure water, indicating its aggregation. Scheme 55. PEGylated porphyrins and chlorins prepared through click chemistry, as described by the group of Lindsey [136]. Scheme 55. PEGylated porphyrins and chlorins prepared through click chemistry, as described by the group of Lindsey [136]. Lindsey and co-workers also used an amide coupling of an alkyl-amine substituted bacteriochlorin with a PEG-NHS ester to produce PEGylated bacteriochlorin 186 (Scheme 57) [135]. The β-functionalized bacteriochlorin 185 was prepared by Sonogashira coupling and subsequent reduction of the alkynes. Bocdeprotection was followed by saponificiation to furnish the amine and acid-derivatized intermediate, which was reacted with a PEG-NHS ester to provide the PEGylated bacteriochlorin 186. The carboxylic acid functionality on this chromophore is available for bioconjugation. Lindsey and co-workers also used an amide coupling of an alkyl-amine substituted bacteriochlorin with a PEG-NHS ester to produce PEGylated bacteriochlorin 186 (Scheme 57) [135]. The β-functionalized bacteriochlorin 185 was prepared by Sonogashira coupling and subsequent reduction of the alkynes. Boc-deprotection was followed by saponificiation to furnish the amine and acid-derivatized intermediate, which was reacted with a PEG-NHS ester to provide the PEGylated bacteriochlorin 186. The carboxylic acid functionality on this chromophore is available for bioconjugation.
Lindsey and co-workers also used an amide coupling of an alkyl-amine substituted bacteriochlorin with a PEG-NHS ester to produce PEGylated bacteriochlorin 186 (Scheme 57) [135]. The β-functionalized bacteriochlorin 185 was prepared by Sonogashira coupling and subsequent reduction of the alkynes. Bocdeprotection was followed by saponificiation to furnish the amine and acid-derivatized intermediate, which was reacted with a PEG-NHS ester to provide the PEGylated bacteriochlorin 186. The carboxylic acid functionality on this chromophore is available for bioconjugation. Scheme 57. PEGylated bacteriochlorins bearing a bioconjugatable tether prepared by amide coupling, as described by the group of Lindsey [135].

Summary and Outlook
In summary, significant progress has been made in the past decades toward the preparation of water-soluble porphyrins and hydroporphyrins. A wide range of options are available for their solubilization in aqueous media. Cationic, anionic or neutral groups may be introduced in regio-and chemoselective fashion. Their number and positioning has major influences on the solubility of the derivatized porphyrin, whereby swallowtail approaches stand out as seemingly particularly effective in mediating water-solubility with a moderate concomitant increase in molecular weight. All solubilizing functionalities can be introduced at early stages of the synthesis of the target compound-generally in protected form-or at late stages. The late-state introduction of the solubilizing motif(s) reduces the number of difficult chromatographic steps needed in the synthetic sequence; and these polar moieties and/or their water-solubility generally complicate their isolation and purification. Irrespective of the timing of the introduction of the solubilizing groups, multiple linking strategies are available. As far as flexibility and ease of implementation, PEGylation strategies stand out because they generate neutral chromophores of good solubility, the PEG chains are chemically stable, the versatility of the linking moieties that can be used to link PEG chains to the chromophore, and the facility of the work-up conditions once the PEG chains are established. A combined approach using both ionic and PEG groups may also have its merits in cases where the introduction of short PEGs was not enough to solubilize the macrocycle.

Summary and Outlook
In summary, significant progress has been made in the past decades toward the preparation of water-soluble porphyrins and hydroporphyrins. A wide range of options are available for their solubilization in aqueous media. Cationic, anionic or neutral groups may be introduced in regio-and chemoselective fashion. Their number and positioning has major influences on the solubility of the derivatized porphyrin, whereby swallowtail approaches stand out as seemingly particularly effective in mediating water-solubility with a moderate concomitant increase in molecular weight. All solubilizing functionalities can be introduced at early stages of the synthesis of the target compound-generally in protected form-or at late stages. The late-state introduction of the solubilizing motif(s) reduces the number of difficult chromatographic steps needed in the synthetic sequence; and these polar moieties and/or their water-solubility generally complicate their isolation and purification. Irrespective of the timing of the introduction of the solubilizing groups, multiple linking strategies are available. As far as flexibility and ease of implementation, PEGylation strategies stand out because they generate neutral chromophores of good solubility, the PEG chains are chemically stable, the versatility of the linking moieties that can be used to link PEG chains to the chromophore, and the facility of the work-up conditions once the PEG chains are established. A combined approach using both ionic and PEG groups may also have its merits in cases where the introduction of short PEGs was not enough to solubilize the macrocycle.
Even though the toolbox for the synthetic chemist to affect water-solubility is already extensive, the continued development of solubilizing strategies that are mild, selective, and introduce chemically robust solubilization motifs to porphyrins is vital to the field for these versatile chromophores to realize their full potential in the many technical and biomedical applications that take place in aqueous media.